Allergen detection agents and assays

ABSTRACT

The present application discloses nucleic acid aptamer based signaling polynucleotides (SPNs) that specifically bind an allergen protein. Provided in the present invention include aptamers, SPNs, SPN-complement complexes, magnetic particle conjugates, DNA printed glass slides and detection agents, and detection methods using the same for detecting the presence, or absence of an allergen protein in a food sample.

CROSS REFERENCE TO RELATED APPLICATION

This application claims priority to U.S. Provisional Application Ser. No. 62/418,984, filed on Nov. 8, 2016; U.S. Provisional Application Ser. No. 62/435,106, filed on Dec. 16, 2016, and U.S. Provisional Application Ser. No. 62/512,299, filed on May 30, 2017; the contents of each of which are incorporated herein by reference in their entirety.

REFERENCE TO THE SEQUENCE LISTING

The present application is being filed along with a Sequence Listing in electronic format. The Sequence Listing is provided as a file entitled 20661007PCTSEQLST.txt, created on Nov. 6, 2017, which is 2,514,969 bytes in size. The information in the electronic format of the sequence listing is incorporated herein by reference in its entirety.

FIELD OF THE INVENTION

The present invention relates to nucleic acid based signaling polynucleotides (SPNs) for detecting allergen proteins. Detection agents comprising SPNs of the present invention can be used as novel biosensor platforms.

BACKGROUND OF THE INVENTION

Allergy is a serious medical condition affecting millions of people worldwide, with about 15 million people in the United States, including many children. During an allergic reaction, the immune system mistakenly targets an allergen as a threat and attacks it. The allergic reaction may affect the skin, the digestive system, the gastrointestinal tract, the respiratory system, the circulatory system and the cardiovascular system; in some allergic reactions, multiple organ systems are affected. Allergic reactions range from mild to severe or life-threatening. Severe symptoms may include difficulty in breathing, low blood pressure, chest pain, loss of consciousness, and anaphylaxis. People having allergies currently manage their allergies by avoiding any food that might contain that specific allergen. These restrictions have a major impact on the patients' quality of life and there remains no method for assessing the true allergen content of food. In the United States, food allergy symptoms send someone to the emergency room every three minutes.

Though antibody-based immunoassays are commonly used for food allergen detection, given the fact that antibodies to allergens are not easily to be obtained, there is an unmet demand of new platform technology to improve in vitro allergen detection in both clinical and non-clinical settings. Nucleic acids, for example, nucleic acid aptamers are promising alternatives or supplements to antibodies for this purpose. These small RNA/DNA molecules can form secondary and tertiary structures capable of specifically binding proteins or other targets. Aptamers can be developed against a seemingly unlimited range of targets such as small inorganic ions, drugs, organic peptides, proteins and even complex cells. Aptamers are thermally stable, so they can be stored and transported easily. These properties make aptamers good agents for analyte detection in a sample, protein/nucleic acid purification and other aspects of biological researches.

Methods using aptamers specific allergen proteins have been reported for detection of several common allergens, for example, gluten (PCT Publication PCT/ES2013/000133 to Amaya-Gonzalez, et al.), and toxic ß-conglutin (Lup an 1) (Nadal, et al., PLoS ONE, 2012, 7(4): e35253; Nadal, et al., Anal. Bioanal. Chem. 2013, 405: 9343-9349; and Mairal, et al., Biosensors and Bioelectronics, 2014, 54: 207-210.) The present inventors have recognized that allergen detection in various matrices of food products can be conveniently performed using aptamer-based detector sequences such as signaling polynucleotides (SPNs), which are particularly well suited for use in a simple and portable sensor that can be used repetitively with high sensitivity and reproducibility at ambient temperature to ensure food safety. Recent patent applications by the inventors disclose allergen specific aptamers, SPNs and their applications in allergen detection, including PCT patent application publication NO.: WO2015/066027; PCT Patent Application Serial NO.: PCT/US 16/29356; and U.S. Patent Application Ser. No. 62/308,377; the contents of each of which are incorporated by reference in their entirety.

In addition to sensitive ligands (e.g., nucleic acid aptamers) that bind analytes of interest (e.g., an allergen protein), materials and surfaces that enhance the analytic performance of the ligands and biosensors are also important. Recently A wide variety of materials including magnetic particles, gold or latex particles and electrode surfaces have been used in many settings as strategies for signaling amplification. The properties of magnetic particles, both nano- and micro-size dimensions, have proved to be promising substrates to be coupled with detection ligands for the design of cost-effective biosensing platforms.

The present application discloses magnetic particle conjugates comprising SPNs and/or SPN complexes that are suitable for allergen detection with high sensitivity and specificity. Such SPN-magnetic particle conjugates may be used as detection agents for allergen detection in a variety of analyte detection assays, kits, devices and systems.

SUMMARY OF THE INVENTION

The present invention provides signaling polynucleotides (SPNs), SPN-complement complexes, magnetic particle conjugates, DNA printed glass slides and detection agents for allergen detection, and biosensors, assays and method for detecting allergen proteins in food samples using the compositions and agents discussed in the present disclosure.

In one embodiment, SPNs derived from nucleic acid aptamers having nucleic acid sequences that bind allergens with high specificity and affinity are provided. In some aspects, the signaling polynucleotides comprise nucleic acid sequences of SEQ ID NOs.: 1-696, which bind specifically to eight common food allergens. In some aspects, the SPN comprises a nucleic acid sequence that specifically binds to cashew selected from SEQ ID NOs.: 1-12. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to peanut selected from SEQ ID NOs.: 13-24, 96 and 97-496. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to tree nut selected from SEQ ID NOs.: 497-696. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to milk selected from SEQ ID NOs.: 25-34. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to fish allergen selected from SEQ ID NOs.: 35-46. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to egg selected from SEQ ID NOs.: 47-58 and 93-94. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to gluten selected from SEQ ID NOs.: 59-70 and 91-92. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to soy allergen selected from SEQ ID NOs.: 71-80. In other aspects, the SPN may comprise a nucleic acid sequence that specifically binds to crustacean selected from SEQ ID NOs.: 81-90.

In one embodiment, SPN-complement complexes are provided in accordance with the present invention. The SPN-complement complex comprises a SPN and a short nucleic acid sequence complementary to a portion of the sequence of the SPN, wherein the SPN and its corresponding complementary sequence are hybridized to form the complex. In one example, the complement is complementary to either the 5′ end or 3′ end sequence of the SPN. In some aspects, the complementary sequence contains about 5-20 nucleotide residues. In one preferred example, the complementary sequence contains 5-10 nucleotide residues.

In one embodiment, magnetic particle conjugates are provided in accordance with the present invention. The magnetic particle conjugates comprise SPN-complement complexes covalently immobilized on the surface of the particles. The magnetic particles may be micro-magnetic particles (MMPs) or nano-magnetic particles (NMPs). In some aspects, the 3′ end of the SPN is linked to magnetic particles, for example, through a 3′ amine or 3′ thiol group, or the addition of a poly-A sequence at the end, or a biotin modification. In other aspects, the 5′ end of the SPN is linked to magnetic particles, for example, through a 5′ amine or 5′ thiol group, or a biotin modification. Accordingly, the complementary sequence contains nucleotide sequences complementary to the free end of the SPN. In further other aspects, the SPN is linked to magnetic particles through its complementary sequence which is covalently immobilized on the surface of magnetic particles. In some examples, the complementary sequence may be attached to the surface of magnetic beads through amine, or thiol, or biotin-streptavidin linkage. In some aspects, magnetic particles may be further coated with PEG polymers or ethanolamine-PEG linkers.

In another embodiment. SPNs and SPN-complement complexes may be attached to the surface of a solid support; such solid support may be a glass slide, a silicon chip or wafer or a microwell plate. The DNA-printed surface may be used as a biosensing platform in a variety of settings for allergen detection. For example, a DNA printed glass slide may be inserted into a detection sensor for detection of a target allergen. In some aspects, one end of the SPN is attached to the two-dimensional surface of the solid support. The complement and allergen protein compete each other for binding to the attached SPN. In other aspects, the short complement is attached to the two-dimensional surface of the solid support. The SPN is hybridized with the complement to form complexes.

The covalent conjugation of nucleic acid molecules of the present invention (e.g., aptamer. SPN and SPN complement) to a surface, either a three-dimensional surface of magnetic particle or a two-dimensional surface of a glass slide can be through a thiol-maleimide mediated covalent chemical reaction, or an amine-mediated reaction, or a biotin-streptavidin linkage. In one example, the surface of a solid substrate (e.g. magnetic particles and glass slides) may be further coated with PEG polymers or ethanolamine-PEG linkers.

In some aspects, the nucleic acid sequence may be directly synthesized in situ on the solid substrate. In one embodiment, the short complementary oligonucleotide is directly synthesized on the solid substrate at a low density. A stable non-cleavable linker and optionally a spacer group may be used for in situ synthetic reaction.

In one embodiment, detection agents comprising SPNs, SPN-complement complexes, magnetic particle conjugates and/or DNA printed solid glasses are provided in accordance with the present invention. The detection agents may be used in any biosensor platform for capturing and detecting allergen proteins in food samples. In some aspects, the agents may be labeled with a fluorescent marker. The fluorescent marker may be conjugated to the agent in a variety of configurations. In one example, one end of the complementary sequence may be labeled with a fluorophore. In this configuration, a target allergen protein when binding to the SPN, will detach the complementary sequence hybridized with the SPN, resulting in “fluorescent signal of”. In another embodiment, one end of the complementary sequence is labeled with a quencher and the free end of the SPN is labeled with a fluorophore. Therefore, the fluorescent signal is quenched in the SPN-complement complex. The binding of a target allergen will detach the complementary sequence hybridized with the SPN, resulting in the quenched fluorescent signal back on. In further another example, one end of the complementary sequence and the free end of the SPN are labeled with different fluorophores. The binding of a target allergen will detach the complementary sequence hybridized with the SPN, resulting in a change in fluorescent signal. In each signal configuration, changes in fluorescent signals can be used to determine the presence and/or absence of the target allergen in food samples.

In accordance with the present invention, kits, biosensors and devices dependent on the present compositions and agents are also provided.

In other embodiments, the present invention provides assays and methods for detecting the presence, absence and/or quantity of an allergen of interest in a sample.

BRIEF DESCRIPTION OF DRAWINGS

FIG. 1A, FIG. 1B and FIG. 1C illustrate configurations of detection agents comprising SPN-complement complexes and magnetic particles. FIG. 1A displays a SPN linked to a magnetic particle through a thiol modification at the 5′end. FIG. 1B display a SPN linked to a magnetic particle through 3′polyA. FIG. 1C displays a SPN linked to a magnetic particle through an amine modification at the 5′end.

FIG. 2A is a representative fluorescent signal measurement of the 5′thiol modification. C1 indicates the complementary sequence is 15 nucleotides in length, while C2 indicates that the complementary sequence is 10 nucleotides in length. FIG. 2B and FIG. 2C are representative signals of the 5′ thiol modification. C3 indicates that the complementary sequence includes 5 complementary nucleotides and 5nt polyA.

FIG. 3 is a diagram showing fluorescence signal off using magnetic beads conjugated with 5′thiol modified Ara H aptamer in foods spiked with different concentrations of peanut.

FIG. 4A, FIG. 4B and FIG. 4C demonstrate fluorescence off; fluorescence on and dual dye configurations of SPN-complement complexes, respectively.

FIG. 5A illustrates a diagram of SPN-complement complexes conjugated to the surface of a solid substrate through one end of the SPN for exposing allergen proteins; FIG. 5B displays a diagram of a complementary sequence conjugated to the surface of a solid substrate for exposing the SPN-allergen complexes.

FIG. 6A demonstrates an attachment assay using the complementary sequence printed glass slide. The SPNs and their allergen proteins are premixed and form SPN-protein complexes. The free SPNs and SPN-protein complexes will compete with each other to attach to the complementary sequences on the surface. FIG. 6B demonstrates a detachment assay. The SPNs are first hybridized with the complementary sequences on the surface, forming SPN-complement complexes. Allergen proteins are added and bind to the SPNs. The SPN-protein complexes detach from the surface and will be washed off.

FIG. 7A is a representative histogram of detection of peanut diluted in buffer. Peanut specific SPNs are conjugated to magnetic beads and fluorescent signals are recorded using a lab grade LED based reader.

FIG. 7B is a representative histogram of detection of peanut spiked in cookie. Peanut specific SPNs are conjugated to magnetic beads and fluorescent signals are recorded using a lab grade LED based reader.

FIG. 8A is a representative histogram of signal reduction when comparing food samples with and without peanut. Peanut specific SPNs are conjugated to magnetic beads and fluorescent signals are recorded using a lab grade LED based e reader.

FIG. 8B is representative histogram showing signal reduction in 5 different food samples spiked with peanut at different concentrations. Peanut specific SPNs are conjugated to magnetic beads and fluorescent signals are recorded using a lab grade LED based reader.

FIG. 9A shows peanut concentration curve in buffer measured on the detection assay with nucleic acid coated solid surface (chip) (N=5, LOD=1.25 ppm peanut).

FIG. 9B shows peanut concentration curve in shortbread cookie measured in the detection assay with nucleic acid coated solid surface (chip) (N=3, LOD=1.25 ppm peanut).

FIG. 10A demonstrates the sensitivity of detection assay with nucleic acid coated solid surface on the rig.

FIG. 10B demonstrates the sensitivity of detection assay with nucleic acid solid surface on the lab-grade bench-top chip.

FIG. 10C is a representative histogram showing that the same detection sensitivity is retained in diverse chocolate matrices in nucleic acid coated chip based assay on the rig.

FIG. 11A demonstrates the detection signal read by the lab-grade LED reader in different food matrices in magnetic bead conjugates based assay. The food samples were prepared using GentleMACS homogenizer and processed by centrifugation.

FIG. 11B demonstrates the detection signal read by the designed optic sensor in different food matrices in solid surface (chip) based assay. The food samples were prepared using GentleMACS homogenizer and processed by centrifugation.

FIG. 11C demonstrates the detection signal read by the lab-grade LED based reader in 5 food matrices in magnetic bead conjugates based assay. The food samples were prepared using designed rotor homogenizer and filtered using 0.2 micron PES filter.

FIG. 11D demonstrates the detection signal read by the designed optic sensor in 9 food matrices in solid surface (chip) based assay. The food samples were prepared using designed rotor homogenizer and filtered using 0.1 micron PES filter.

FIG. 12 demonstrates the effect of decreased reaction volume on detection sensitivity.

FIG. 13A is a representative diagram of the control panels and detection area (unknown) on the chip. FIG. 13B is a representative signal reading of the chip. FIG. 13C demonstrate a representative control signal measurement.

FIG. 14A depicts the effect of MgCl2 when added to the extraction buffer. FIG. 14B depicts the effect of MgCl2 when added after extraction and filtration. FIG. 14C is a representative reading of detection signals with various concentrations of MgCl2.

FIG. 15 shows the sensitivity in solid surface assays with optimized conditions and reduced reaction time.

FIGS. 16A to 16D demonstrate the stability of reaction agents including SPNs and extraction buffer.

DETAILED DESCRIPTION OF THE INVENTION

The details of one or more embodiments of the invention are set forth in the accompanying description below. Although any materials and methods similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred materials and methods are now described. Other features, objects and advantages of the invention will be apparent from the description. In the description, the singular forms also include the plural unless the context clearly dictates otherwise. Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. In the case of conflict, the present description will control.

I. Compositions of the Present Invention

The present invention provides compositions, conjugates and detection agents for allergen detection. The functional/core component of a detection agent is a nucleic acid aptamer that specifically binds an allergen protein. In accordance with the present invention, an allergen specific aptamer may be modified to form a signal polynucleotide (SPN) (described in detail herein below). The SPN may be used as a free detection agent, or conjugated to a particle or a solid surface as a complex detection agent. In some aspects, the SPNs alone work as both binding ligands and signaling molecules or labels. In other aspects, complexes composed of SPNs and their complementary sequences work as both binding ligands and signaling molecules or labels. Aptamers, SPNs and/or SPN-complement complexes can be conjugated to any particles such as metal nanoparticles, redox compounds and magnetic particles, magnetic microparticles, and other solid surfaces such as glass slides and silicon chips, forming biosensor platforms.

Aptamers comprising nucleic acid sequences that bind common food allergens are isolated through SELEX selections. Aptamers are then modified to generate signal polynucleotides (SPNs) which work as capturing and detecting ligands for allergen proteins. In particular, the SPN may comprise a nucleic acid sequence selected from SEQ ID NOs.: 1-696.

In some aspects, the SPN comprises a nucleic acid sequence that specifically binds to cashew selected from SEQ ID NOs.: 1-12; the cashew specific SPN has a unique sequence of SEQ ID. NOs.: 1-6. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to peanut selected from SEQ ID NOs.: 13-24, and 96-696; the peanut specific SPN has a unique sequence of SEQ ID NOs.: 13-18 and 97-296. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to tree nut selected from SEQ ID NOs.: 497-696; the tree nut specific SPN has a unique sequence of SEQ ID NOs.: 497-596. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to milk selected from SEQ ID NOs.: 25-34; the milk specific SPN has a unique sequence of SEQ ID NOs.: 25-29. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to fish allergen selected from SEQ ID NOs.: 35-46; the fish specific SPN has a unique sequence of SEQ ID NOs.: 35-40. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to egg selected from SEQ ID NOs.: 47-58 and 93-94; the egg specific SPN has a unique sequence of SEQ ID NOs.: 47-52. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to gluten selected from SEQ ID NOs.: 59-70 and 91-92, the gluten specific SPN has a unique sequence of SEQ ID NOs.: 59-64. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to soy allergen selected from SEQ ID NOs.: 71-80; the soy specific SPN has a unique sequence of SEQ ID NOs.: 71-75. In other aspects, the SPN may comprise a nucleic acid sequence that specifically binds to crustacean selected from SEQ ID NOs.: 81-90; the crustacean specific SPN has a unique sequence of SEQ ID NOs.: 81-85.

In some embodiments, a SPN and a short nucleic acid sequence which is complementary to a portion of the sequence of the SPN (e.g., the sequence at either the 5′ end or 3′ end of the SPN) may be hybridized to form a complex (referred to “SPN-complement complex”). The SPN-complement complexes may be attached to the surface of magnetic particles or other solid surfaces through either the SPN or the complementary sequence.

In some embodiments, SPNs of the present invention are conjugated to the surface of magnetic particles or a solid substrate (e.g., a glass slide) at one end, e.g. the 5′ end or 3′end (e.g., as shown in FIGS. 4A, 4B and 4C and FIG. 5A). Nucleic acid molecules can be covalently attached to magnetic particles/beads by methods based on the formation of covalent bonds. Carboxyl and amino groups are the most common reactive groups for attaching ligands to surfaces. In some aspects, a primary amine (—NH2) modifier may be placed to the 5′end, or 3′end of a nucleic acid molecule (e.g., SPN), or internally using an amino-C or amino-T modified base. The amino-modified nucleic acid molecules may be attached to magnetic particles using an acylating reagent, for example Carbodiimide (EDC). In other aspects, a thiol group (—SH) may be attached to the 5′ or 3′ end of a nucleic acid molecule (e.g., a SPN). The thiol (—SH) modifier enables covalent attachment of a nucleic acid molecule to a variety of substrates including magnetic particles, via disulfide bond (—S—S—) or maleimide linkages. In another example, a biotinylated SPN may be conjugated to streptavidin-coated magnetic particles. In another example, PEG polymers may be introduced to the surface of a solid substrate before the conjugation.

In this context, the opposite end of the SPN which is free from the attached magnetic particles may be hybridized with the complementary sequence, forming a SPN-complement complex. The short complementary sequences may be labeled with a fluorescent dye, such as Alex 647, Cy5, Cy3-FITC and Texas red. The binding of an allergen to the SPN will detach the complementary sequence from the complex, resulting in a signaling change (as shown in FIG. 5A).

In some embodiments, the complementary sequences of the SPNs may be conjugated to the surface of magnetic particles or other solid substrates (e.g., printed glass surface) through covalent bindings as discussed herein. In this context, the printed glass surface having such complementary sequences may be exposed to the SPNs and allergen proteins. In this context, either an attachment assay or detachment assay may be developed for detection of allergen proteins (FIG. 6A and FIG. 6B). For example, in the attachment assay, the SPNs and allergen proteins are premixed before being exposed to the complementary sequences. Only the free SPNs will bind to the complements (FIG. 5B and FIG. 6A), generating fluorescent signals from the fluorescent dye at either the 5′end or 3′end of the SPN. As non-limiting examples, the fluorophore may be selected from Alex Fluor® fluorophores (such as Alex 514, Alex 532, Alex 546, Alex 555, Alex 568, Alex 594, Alex 610, Alex 633, Alex 635, Alex 647, Alex 660, Alex 680, Alexa 700, Alex 750, Alex 800, Alex 610-R-phycoerythrin (R-PE), Alex 647-R-phycoerythrin (R-PE), Alex 680-R-phycoerythrin (R-PE), and Alex 680-Allophycocyanin (APC)), Allophycocyanin (APC) and its derivatives, Cy fluorophores (e.g., Cy3.5, Cy3-FITC, CY5, CY 5.5, CY7, CY7-APC, CY5.5-APC), Qdots, TRITC, R-PE, Tamara, Rhodamine Red-X, Rox, TruRed, SYPRO red, BODIPY TR, Propidium iodide and Texas red. In some examples, the fluorescent dye is Alex 647, Cy5, CY3-FITC or Texas red.

In other embodiments, nucleic acid molecules of the present invention may be attached to solid surfaces by in situ oligonucleotide synthesis.

Aptamers, Signaling Polynucleotides (SPNs) and SPN-Complement Complex

Aptamers (sometimes also called chemical antibodies) are single-stranded oligonucleotides (RNA or single stranded DNA) that form stable but unique three-dimensional confirmations capable of binding with high affinity and specificity to a variety of molecular targets. Aptamers bind to protein targets in much the same manner as antibodies and modulate protein function. Thus, aptamers are also referred to as “chemical antibodies”. Aptamers have advantages over antibodies in that they are poorly immunogenic, stable, and often bind to a target molecule more strongly than do antibodies. Generally aptamers can be synthesized easily and in large quantities by in vitro transcription, PCR, or chemical synthesis (Annu. Rev. Med. 2005, 56, 555-583; Nat. Rev. Drug Discov. 2006, 5, 123-132), and target-specific aptamers can be selected from random-sequence, single-stranded nucleic acid libraries by an in vitro selection and amplification procedure known as SELEX (systematic evolution of ligands by exponential enrichment). The selected aptamers are small single-stranded nucleic acids that fold into a well-defined three-dimensional structure. They show a high affinity and specificity for their target molecules and inhibit their biological functions. Furthermore, aptamers have important properties that simplify its industrialization. For example, aptamers are thermally stable, so they can be stored and transported easily. Aptamers can be produced or modified in large scale, with minimal batch-to-batch variation, given the well-established chemical synthesis and modification technologies.

Aptamers are useful and cost-effective tools for biochemical analyses. Also, they can be developed quickly against a seemingly unlimited range of targets. To date, specific aptamers against diverse targets have been successfully developed, including small inorganic irons, organic peptides, drugs, proteins, lipids and even complex cells. One of the more recent reviews of aptamer-based analysis in context of food safety control indicated that the selection of aptamers for this group of ingredients is emerging (Amaya-Gonzalez et al., Sensors 2013, 13: 16292-16311, the contents of which are incorporated herein by reference in its entirety).

1. Selection of Aptamers Specific to a Target

Aptamers can be artificially generated by a method called systematic evolution of ligands by exponential enrichment (SELEX) (Tuerk and Gold, Science, 1990, 249, 505-510). More recently, a new improved separation technology for aptamer selection was introduced, capillary electrophoresis (CE)-SELEX (Mosing and Bowser, Methods Mol Biol., 2009, 535: 33-43).

Aptamers that bind to virtually any particular target can be selected by using an iterative process called SELEX™ (Systemic Evolution of Ligands by Exponential Enrichment). The process is described in, for example U.S. Pat. Nos. 5,270,163 and 5,475,096. The SELEX™ process is based on the unique insight that nucleic acids have sufficient capacity for forming a variety of two- and three-dimensional structures and sufficient chemical versatility available within their monomers to act as ligands (i.e., form specific binding pairs) with virtually any chemical compound, whether monomeric or polymeric.

The SELEX™ process relies, as a starting point, upon a large library or pool of single stranded oligonucleotides comprising randomized sequences. The oligonucleotides can be modified or unmodified DNA, RNA, or DNA/RNA hybrids. In some examples, the pool comprises 100% random or partially random oligonucleotides. In other examples, the pool comprises random or partially random oligonucleotides containing at least one fixed sequence and/or conserved sequence incorporated within randomized sequence. In other examples, the pool comprises random or partially random oligonucleotides containing at least one fixed sequence and/or conserved sequence at its 5′ and/or 3′ end which may comprise a sequence shared by all the molecules of the oligonucleotide pool. Fixed sequences are sequences common to oligonucleotides in the pool which are incorporated for a preselected purpose such as, CpG motifs, hybridization sites for PCR primers, promoter sequences for RNA polymerases (e.g., T3, T4, T7, and SP6), restriction sites, or homopolymeric sequences, such as poly A or poly T tracts, catalytic cores, sites for selective binding to affinity columns, and other sequences to facilitate cloning and/or sequencing of an oligonucleotide of interest. Conserved sequences are sequences, other than the previously described fixed sequences, shared by a number of aptamers that bind to the same target.

The oligonucleotides of the pool preferably include a randomized sequence portion as well as fixed sequences necessary for efficient amplification. Typically, the oligonucleotides of the starting pool contain fixed 5′ and 3′ terminal sequences which flank an internal region of 30-50 random nucleotides. The randomized nucleotides can be produced in a number of ways including chemical synthesis and size selection from randomly cleaved cellular nucleic acids. Sequence variation in the test nucleic acids can also be introduced or increased by mutagenesis before or during the selection/amplification iterations.

The random sequence portion of the oligonucleotide can be of any length and can comprise ribonucleotides and/or deoxyribonucleotides and can include modified or non-natural nucleotides or nucleotide analogs (see for example U.S. Pat. Nos. 5,958,691 and 5,660,985). Random oligonucleotides can be synthesized from phosphodiester-linked nucleotides using solid phase oligonucleotide synthesis techniques well known in the art. Random oligonucleotides can also be synthesized using solution phase methods such as triester synthesis methods. Typical syntheses carried out on automated DNA synthesis equipment yield 10¹⁴-10¹⁶ individual molecules, a number sufficient for most SELEX™ experiments.

The starting library of oligonucleotides may be generated by automated chemical synthesis on a DNA synthesizer. Partially random sequences can be created by adding the four nucleotides in different molar ratios at each addition step.

The library of oligonucleotides for aptamer selection may be either RNA or DNA. A RNA library of oligonucleotides is typically generated by transcribing a DNA library of oligonucleotides in vitro using T7 RNA polymerase or modified T7 RNA polymerases and purified. The RNA or DNA library is then mixed with the target under conditions favorable for binding and subjected to step-wise iterations of binding, partitioning and amplification, using the same general selection scheme, to achieve the desired criterion of binding affinity and selectivity as defined in the present application.

More specifically, starting with a mixture containing the starting pool of nucleic acids, the SELEX™ method includes steps of: (a) contacting the mixture with the target under conditions favorable for binding; (b) partitioning unbound nucleic acids from those nucleic acids which have bound specifically to target molecules; (c) dissociating the nucleic acid-target complexes; (d) amplifying the nucleic acids dissociated from the nucleic acid-target complexes to yield a ligand-enriched mixture of nucleic acids; and (e) reiterating the steps of binding, partitioning, dissociating and amplifying through as many cycles as desired to yield highly specific, high affinity nucleic acid ligands to the target molecule. Cycles of selection and amplification are repeated until a desired goal is achieved. Generally this is until no significant improvement in binding strength is achieved on repetition of the cycle. Typically, nucleic acid aptamer molecules are selected in a 5 to 20 cycle procedure.

A variety of nucleic acid primary, secondary and tertiary structures are known to exist. The structures or motifs that have been shown most commonly to be involved in non-Watson-Crick type interactions are referred to as hairpin loops, symmetric and asymmetric bulges, pseudoknots and myriad combinations of the same. The core SELEX™ method has been modified to achieve a number of specific objectives, such as selection of aptamers with particular secondary structures. Examples of SELEX processes can be found in U.S. Pat. Nos. 5,270,163 and 5,475,096. For example, U.S. Pat. No. 5,707,796 describes the use of SELEX™ in conjunction with gel electrophoresis to select nucleic acid molecules with specific structural characteristics, such as bent DNA. U.S. Pat. No. 5,763,177 describes SELEX™ based methods for selecting nucleic acid ligands containing photo reactive groups capable of binding and/or photo-crosslinking to and/or photo-inactivating a target molecule U.S. Pat. Nos. 5,567,588 and 5,861,254 describe SELEX™ based methods which achieve highly efficient partitioning between oligonucleotides having high and low affinity for a target molecule. U.S. Pat. No. 5,496,938 describes methods for obtaining improved nucleic acid ligands after the SELEX™ process has been performed. U.S. Pat. No. 5,705,337 describes methods for covalently linking a ligand to its target, the contents of each of which are incorporated herein by reference in their entirety.

Counter-SELEX™ is a method for improving the specificity of nucleic acid ligands to a target molecule by eliminating nucleic acid ligand sequences with cross-reactivity to one or more non-target molecules. Counter-SELEX™ is comprised of the steps of: (a) preparing a candidate mixture of nucleic acids; (b) contacting the candidate mixture with the target, wherein nucleic acids having an increased affinity to the target relative to the candidate mixture may be partitioned from the remainder of the candidate mixture; (c) partitioning the increased affinity nucleic acids from the remainder of the candidate mixture; (d) dissociating the increased affinity nucleic acids from the target; (e) contacting the increased affinity nucleic acids with one or more non-target molecules such that nucleic acid ligands with specific affinity for the non-target molecule(s) are removed; and (f) amplifying the nucleic acids with specific affinity only to the target molecule to yield a mixture of nucleic acids enriched for nucleic acid sequences with a relatively higher affinity and specificity for binding to the target molecule. As described above for SELEX™, cycles of selection and amplification are repeated as necessary until a desired goal is achieved.

The binding affinity describes the measure of the strength of the binding or affinity of molecules to each other. Binding affinity of the aptamer herein with respect to targets and other molecules is defined in terms of K_(d). The dissociation constant can be determined by methods known in the art. It has been observed, however, that for some small oligonucleotides, direct determination of K_(d) is difficult, and can lead to misleadingly high results. Under these circumstances, a competitive binding assay for the target molecule or other candidate substance can be conducted with respect to substances known to bind the target or candidate. The value of the concentration at which 50% inhibition occurs (K_(s)) is, under ideal conditions, equivalent to K_(d).

In accordance with the present invention, a SELEX approach was used to select core binding aptamers that bind 8 major food allergens (i.e. cashew, egg, milk, peanuts, gluten, fish, crustacean and soy). Several aptamers with sequences that can specifically recognize a target allergen were selected and the nucleic acid sequences of selected aptamers were further modified to generate signaling polynucleotides. The aptamers with high selectivity, specificity and stability are selected and further labeled as detection agents. The sequences of the selected aptamers for the 8 major allergens are listed in Table 1. For example, an aptamer having a full sequence (SEQ ID NO.: 7) is one of the SPNs that bind cashew. The full sequence includes the primers used for the screen and the core binding sequence of the aptamer (SEQ ID NO.: 1), the full sequence will be further modified to generate signaling polynucleotides (SPNs) specific to cashew, as discussed herein below.

2. Aptamer Modifications

In accordance with the present invention, oligonucleotides and aptamers may be further modified to improve their stability. The present invention also includes analogs as described herein and/or additional modifications designed to improve one or more characteristics of aptamers such as protection from nuclease digestion. Oligonucleotide modifications contemplated in the present invention include, but are not limited to, those which provide other chemical groups that incorporate additional charge, polarizability, hydrophobicity, hydrogen bonding, electrostatic interaction, and fluxionality to the nucleic acid ligand bases or to the nucleic acid ligand as a whole.

Modifications to generate oligonucleotides which are resistant to nucleases can also include one or more substitute internucleotide linkages, altered sugars, altered bases, or combinations thereof. Such modifications include 2′-position sugar modifications, 5-position pyrimidine modifications, 8-position purine modifications, modifications at exocyclic amines, substitution of 4-thiouridine, substitution of 5-bromo or 5-iodo-uracil, backbone modifications, phosphorothioate or alkyl phosphate modifications, methylations, and unusual base-pairing combinations such as the isobases isocytidine and isoguanosine, 3′ and 5′ modifications such as capping; conjugation to a high molecular weight, non-immunogenic compound; conjugation to a lipophilic compound; and phosphate backbone modification.

Nucleic acid aptamers may be ribonucleic acid, deoxyribonucleic acid, or mixed ribonucleic acid and deoxyribonucleic acid. Aptamers may be single stranded ribonucleic acid, deoxyribonucleic acid or mixed ribonucleic acid and deoxyribonucleic acid.

Nucleic acid aptamers comprise a series of linked nucleosides or nucleotides. The term “nucleic acid,” in its broadest sense, includes any compound and/or substance that comprise a polymer of nucleotides. These polymers are often referred to as polynucleotides. Exemplary nucleic acid molecules or polynucleotides of the invention include, but are not limited to, either D- or L-nucleic acids, ribonucleic acids (RNAs), deoxyribonucleic acids (DNAs), threose nucleic acids (TNAs), glycol nucleic acids (GNAs), peptide nucleic acids (PNAs), locked nucleic acids (LNAs, including LNA having a β-D-ribo configuration, α-LNA having an α-L-ribo configuration (a diastereomer of LNA), 2′-amino-LNA having a 2′-amino functionalization, and 2′-amino-α-LNA having a 2′-amino functionalization) or hybrids thereof.

The skilled artisan will recognize that the term “RNA molecule” or “ribonucleic acid molecule” encompasses not only RNA molecules as expressed or found in nature, but also analogs and derivatives of RNA comprising one or more ribonucleotide/ribonucleoside analogs or derivatives as described herein or as known in the art. Strictly speaking, a “ribonucleoside” includes a nucleoside base and a ribose sugar, and a “ribonucleotide” is a ribonucleoside with one, two or three phosphate moieties. However, the terms “ribonucleoside” and “ribonucleotide” can be considered to be equivalent as used herein. The RNA can be modified in the nucleobase structure, the ribofuranosyl ring or in the ribose-phosphate backbone.

In some embodiments, the aptamer comprises at least one chemical modification. In some embodiments, the chemical modification is selected from a chemical substitution of the nucleic acid at a sugar position, a chemical substitution at a phosphate position and a chemical substitution at a base position. In other embodiments, the chemical modification is selected from incorporation of a modified nucleotide; 3′ capping; conjugation to a high molecular weight, non-immunogenic compound; conjugation to a lipophilic compound; and incorporation of phosphorothioate into the phosphate backbone. In a preferred embodiment, the high molecular weight, non-immunogenic compound is polyalkylene glycol, and more preferably is polyethylene glycol (PEG). The process of covalent conjugation of PEG to another molecule, normally a drug or therapeutic protein is known as PEGylation. PEGylation is routinely achieved by incubation of a reactive derivative of PEG with the target molecule. The covalent attachment of PEG to a drug or therapeutic protein can mask the agent from the host's immune system, thereby providing reduced immunogenicity and antigenicity, and increase the hydrodynamic size (size in solution) of the agent which prolongs its circulatory time by reducing renal clearance. PEGylation can also provide water solubility to hydrophobic drugs and proteins.

In another preferred embodiment, the 3′ cap is an inverted deoxythymidine cap.

In some embodiments, nucleic acid aptamers are provided in which the P(O)O group is replaced by P(O)S (“thioate”), P(S)S (“dithioate”). P(O)NR2 (“amidate”), P(O)R, P(O)OR′, CO or CH2 (“formacetal”) or 3′-amine (—NH—CH2-CH2-), wherein each R or R′ is independently H or substituted or unsubstituted alkyl. Linkage groups can be attached to adjacent nucleotide through a —O—, —N—, or —S— linkage. Not all linkages in the nucleic acid aptamers are required to be identical.

As non-limiting examples, a nucleic acid aptamer can include D-ribose or L-ribose nucleic acid residues and can also include at least one modified ribonucleoside including but not limited to a 2′-O-methyl modified nucleoside, a nucleoside comprising a 5′ phosphorothioate group, a terminal nucleoside linked to a cholesteryl derivative or dodecanoic acid bisdecylamide group, a locked nucleoside, an abasic nucleoside, an inverted deoxynucleoside or inverted ribonucleoside, a 2′-deoxy-2′-fluoro-modified nucleoside, a 2′-amino-modified nucleoside, a 2′-alkyl-modified nucleoside, a morpholino nucleoside, a phosphoramidate or a non-natural base comprising nucleoside, or any combination thereof. Alternatively, a nucleic acid aptamer can comprise at least two modified ribonucleosides, at least 3, at least 4, at least 5, at least 6, at least 7, at least 8, at least 9, at least 10, at least 15, at least 20 or more modified ribonucleosides, up to the entire length of the molecule. The modifications need not be the same for each of such a plurality of modified deoxy- or ribonucleosides in a nucleic acid molecule.

Aptamer may comprise modified nucleobase (often referred to in the art simply as “base”) for increasing the affinity and specificity for their target protein. As used herein, “unmodified” or “natural” nucleobases include the purine bases adenine (A) and guanine (G), and the pyrimidine bases thymine (T), cytosine (C) and uracil (U). For example, the modified base may be a pyrimidine modified by a hydrophobic group, such as benzyl group, a naphthyl group, or a pyrrolebenzyl group, at its 5-position. Modified nucleoside may be exemplified as 5-(N-benzylcarboxyamide)-2′-deoxyuridine (called BzdU), 5-(N-naphthylcarboxyamide)-2′-deoxyuridine (called NapdU), 5-(N-4-pyrrolebenzyl carboxyamide)-2′-deoxyuridine (called 4-PBdU), 5-(N-benzylcarboxyamide)-2′-deoxycytidine (called BzdC), 5-(N-naphthylcarboxyamide)-2′-deoxycytidine (called NapdC), 5-(N-4-pyrrolebenzylcarboxyamide)-2′-deoxycytidine (called 4-PBdC), 5-(N-benzylcarboxyamide)-2′-uridine (called BzU), 5-(N-naphthylcarboxyamide)-2′-uridine (called NapU), 5-(N-4-pyrrolebenzylcarboxyamide)-2′-uridine (called 4-PBU), 5-(N-benzylcarboxyamide)-2′-cytidine (called BzC), 5-(N-naphthylcarboxyamide)-2′-cytidine (called NapC), 5-(N-4-pyrrolebenzyl carboxyamide)-2′-cytidine (called 4-PBC), and the like, but not be limited thereto. Further nucleobases include those disclosed in U.S. Pat. No. 3,687,808, those disclosed in Modified Nucleosides in Biochemistry, Biotechnology and Medicine, Herdewijn, P. ed. Wiley-VCH, 2008; those disclosed in The Concise Encyclopedia Of Polymer Science And Engineering, pages 858-859, Kroschwitz, J. L, ed. John Wiley & Sons, 1990, those disclosed by Englisch et al., Angewandte Chemie, International Edition, 1991, 30, 613, and those disclosed by Sanghvi, Y S., Chapter 15, dsRNA Research and Applications, pages 289-302, Crooke, S. T. and Lebleu, B., Ed., CRC Press, 1993.

In accordance with the present invention, a suitable nucleotide length for an aptamer ranges from about 15 to about 100 nucleotides (nt), and in various other preferred embodiments, 15-30 nt, 20-25 nt, 30-100 nt, 30-60 nt, 25-70 nt, 25-60 nt, 40-60 nt, 25-40 nt, 30-40 nt, any of 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29, 30, 31, 32, 33, 34, 35, 36, 37, 38, 39 or 40 nt or 40-70 nt in length. In some embodiments, an aptamer may be 41, 42, 43, 44, 45, 46, 47, 48, 49, 50, 51, 52, 53, 54, 55, 56, 57, 58, 59, 60, 61, 62, 63, 64, 65, 66, 67, 68, 69, or 70 nt in length. In other embodiments, an aptamer may 71, 72, 73, 74, 75, 76, 77, 78, 79, 80, 81, 82, 83, 84, 85, 86, 87, 88, 89, 90, 91, 92, 93, 94, 95, 96, 97, 98, 99 or 100 nt in length. However, the sequence can be designed with sufficient flexibility such that it can accommodate interactions of aptamers with two targets at the distances described herein.

In some embodiments, the nucleic acid aptamer comprises one or more regions of double-stranded character. Such double stranded regions may arise from internal self-complementarity or complementarity with a second or further aptamers or oligonucleotide molecule. In some embodiments the double stranded region may be from 4-12, 4-10, 4-8 base pairs in length. In some embodiments the double stranded region may be 5, 6, 7, 8, 9, 10, 11 or 12 base pairs. In some embodiments the double stranded region may form a stem region. Such extended stem regions having double stranded character can serve to stabilize the nucleic acid aptamer. As used herein, the term “double stranded character” means that over any length of two nucleic acid molecules, their sequences form base pairings (standard or nonstandard) of more than 50 percent of the length.

Aptamers may be further modified to provide protection from nuclease and other enzymatic activities. The aptamer sequence can be modified by any suitable methods known in the art. For example, phosphorothioate can be incorporated into the backbone, and 5′-modified pyrimidine can be included in 5′ end of ssDNA for DNA aptamers. For RNA aptamers, modified nucleotides such as substitutions of the 2′-OH groups of the ribose backbone, e.g., with 2′-deoxy-NTP or 2′-fluoro-NTP, can be incorporated into the RNA molecule using T7 RNA polymerase mutants. The resistance of these modified aptamers to nuclease can be tested by incubating them with either purified nucleases or nuclease from mouse serum, and the integrity of aptamers can be analyzed by gel electrophoresis.

In some embodiments, such modified nucleic acid aptamers may be synthesized entirely of modified nucleotides, or with a subset of modified nucleotides. The modifications can be the same or different. All nucleotides may be modified, and all may contain the same modification. All nucleotides may be modified, but contain different modifications, e.g., all nucleotides containing the same base may have one type of modification, while nucleotides containing other bases may have different types of modifications. For example, all purine nucleotides may have one type of modification (or are unmodified), while all pyrimidine nucleotides have another, different type of modification (or are unmodified). In this way, oligonucleotides, or libraries of oligonucleotides are generated using any combination of modifications as disclosed herein.

Aptamers may be either monovalent or multivalent. Aptamers may be monomeric, dimeric, trimeric, tetrameric or higher multimeric. Individual aptamer monomers may be linked to form multimeric aptamer fusion molecules. As a non-limiting example, a linking oligonucleotide (i.e., linker) may be designed to contain sequences complementary to both 5′-arm and 3′-arm regions of random aptamers to form dimeric aptamers. For trimeric or tetrameric aptamers, a small trimeric or tetrameric (i.e., a Holiday junction-like) DNA nanostructure will be engineered to include sequences complementary to the 3′-arm region of the random aptamers, therefore creating multimeric aptamer fusion through hybridization. In addition, 3 to 5 or 5 to 10 dT rich nucleotides can be engineered into the linker polynucleotides as a single stranded region between the aptamer-binding motifs, which offers flexibility and freedom of multiple aptamers to coordinate and synergize multivalent interactions with cellular ligands or receptors. Alternatively, multimeric aptamers can also be formed by mixing biotinylated aptamers with streptavidin.

As used herein, the term “multimeric aptamer” or “multivalent aptamer” refers to an aptamer that comprises multiple monomeric units, wherein each of the monomeric units can be an aptamer on its own. Multivalent aptamers have multivalent binding characteristics. A multimeric aptamer can be a homomultimer or a heteromultimer. The term “homomultimer” refers to a multimeric aptamer that comprises multiple binding units of the same kind, i.e., each unit binds to the same binding site of the same target molecule. The term “heteromultimer” refers to a multimeric aptamer that comprises multiple binding units of different kinds, i.e., each binding unit binds to a different binding site of the same target molecule, or each binding unit binds to a binding site on different target molecule. Thus, a heteromultimer can refer to a multimeric aptamer that binds to one target molecule at different binding sties or a multimeric aptamer that binds to different target molecules. A heteromultimer that binds to different target molecules can also be referred to as a multi-specific multimer.

According to certain embodiments of the present invention, variants and derivatives of aptamers are provided. The term “derivative” is used synonymously with the term “variant” and refers to a molecule that has been modified or changed in any way relative to a reference or starting aptamer. The nucleic acid sequence of aptamer variants may possess substitutions, deletions, and/or insertions at certain positions within the nucleotide sequence, as compared to a reference or starting sequence. Ordinarily, variants will possess at least about 50% identity (homology) to a reference sequence, and preferably, they will be at least about 80%, more preferably at least about 90% identical (homologous) to a reference sequence.

In some embodiments, variant mimics of aptamers of the present invention are provided. As used herein, the term “variant mimic” is one which contains one or more nucleic acids which would mimic an activated sequence. The nucleic acid sequences of variant mimics may comprise naturally occurring nucleic acids, or alternatively, non-naturally occurring nucleic acids.

3. Signaling Polynucleotides (SPNs)

Aptamers selected through the process mentioned above herein may be used as signaling polynucleotides (SPNs) for detection of target allergens. Signaling polynucleotides based on aptamer core/binding sequences are advantageous with respect to the objective of development of simple, yet effective detection assays for biomolecule sensors. In accordance with the present invention, a signaling polynucleotide may be developed from the selected aptamers which specifically bind a target allergen molecule. The polynucleotide sequences are detectable when bound at high affinity and specificity to molecular targets.

In some embodiments, signaling polynucleotides (SPNs) of the present invention comprise the core binding sequences which determine the specificity and affinity of SPNs to a target allergen molecule. The full sequence of a selected aptamer can be shortened by deleting the primers used for aptamer selection without impacting the binding sequence to a target allergen. Additional nucleotides may also be added at the 5′terminus and/or the 3′ terminus, without impacting the binding (core) sequence of each aptamer. 3D structures of such SPNs are predicted using standard structure prediction software. The resulting polynucleotide may form a stable 3D structure. In other aspects, nucleotides added at the termini may increase the stability of the polynucleotide and facilitate magnetic particle conjugation, and/or other modifications. For example, a short polyA sequence may be added to the terminus of a SPN to increase the distance between the SPN and magnetic particles (or other solid surface). The length and sequence of additional nucleotides may vary in the context of the core binding sequence of a signaling polynucleotide. SPNs generated from aptamers against common allergens are listed in Tables 1-4.

In some aspects, the SPN comprises a nucleic acid sequence that specifically binds to cashew selected from SEQ ID NOs.: 1-12; the cashew specific SPN has a unique sequence of SEQ ID. NOs.: 1-6. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to peanut selected from SEQ ID NOs.: 13-24, and 97-496; the peanut specific SPN has a unique sequence of SEQ ID NOs.: 13-18 and 97-296. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to tree nut selected from SEQ ID NOs.: 497-696; the tree nut specific SPN has a unique sequence of SEQ ID NOs.: 497-596. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to milk selected from SEQ ID NOs.: 25-34; the milk specific SPN has a unique sequence of SEQ ID NOs.: 25-29. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to fish allergen selected from SEQ ID NOs.: 35-46; the fish specific SPN has a unique sequence of SEQ ID NOs.: 35-40. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to egg selected from SEQ ID NOs.: 47-58 and 93-94; the egg specific SPN has a unique sequence of SEQ ID NOs.: 47-52. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to gluten selected from SEQ ID NOs.: 59-70 and 91-92; the gluten specific SPN has a unique sequence of SEQ ID NOs.: 59-64. In some aspects, the SPN may comprise a nucleic acid sequence that specifically binds to soy allergen selected from SEQ ID NOs.: 71-80; the soy specific SPN has a unique sequence of SEQ ID NOs.: 71-75. In other aspects, the SPN may comprise a nucleic acid sequence that specifically binds to crustacean selected from SEQ ID NOs.: 81-90; the crustacean specific SPN has a unique sequence of SEQ ID NOs.: 81-85.

TABLE 1 Aptamers and SPNs that bind common allergens SEQ ID NO. Core sequence (5′-3′) SEQ ID NO. Full Sequence (5′-3′) Cashew  1 GCACACCACGTCAAAAATCATTGTCACC  7 TAATACGACTCACTATAGGCGTAGCCTGATGAGGC ACGAAGC ACACCACGTCAAAAATCATTGTCACCACGAAGCCG AAACGTGGTGAAAGCCACGTAGCTGCGCC  2 TGCGCAACATAAGTCTCTTGAAAGACCA  8 TAATACGACTCACTATAGGCGTAGCCTGATGAGTG CGTTCAA CGCAACATAAGTCTCTTGAAAGACCACGTTCAACG AAACGTGGTGAAAGCCACGTAGCTGCGCC  3 CACCCACCATACCAGAAATGTTGACACC  9 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA ACGTGGA CCCACCATACCAGAAATGTTGACACCACGTGGACG AAACGTGGTGAAAGCCACGTAGCTGCGCC  4 TGCACAATGTAATTATCAAAATACACCA 10 TAATACGACTCACTATAGGCGTAGCCTGATGAGTG CGGTTGC CACAATGTAATTATCAAAATACACCACGTTGGCCG AAACGTGGTGAAAGCCACGTAGCTGCGCC  5 CCACATCGTGCAATGCCCGAAACATACC 11 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC ACGTAGA ACATCGTGCAATGCCCGAAACATACCACGTAGACG AAACGTGGTGAAAGCCACGTAGCTGCGCC  6 CTATGCAGTGATGATTAAAGATACCACC 12 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT ACGTGAG ATGCAGTGATGATTAAAGATACCACCACGTGAGCG AAACGTGGTGAAAGCCACGTAGCTGCGCC Peanut 13 CAAATAGTTACAAACACCACGTAG 19 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA AATAGTTACAAACACCACGTAGCGAAACGTGGTGA AAGCCACGTAGCTGCGCC 14 CCCAACTGTACAGTACACCACGTAG 20 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC CAACTGTACAGTACACCACGTAGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 15 CACACACACATTCCACCACGTCACG 21 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA CACACACATTCCACCACGTCACGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 16 CACACGTTACCACACCACGTTGACG 22 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA CACGTTACCACACCACGTTGACGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 17 CGTGCCCGAAACACACACCACGATG 23 TAATACGACTCACTATAGGCGTAGCCTGATGAGCG TGCCCGAAACACACACCACGATGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 18 CTCACCACATACCATGTACCACGTG 24 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT CACCACATACCATGTACCACGTGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC Milk 25 TTCACTGGCTGCACCCACCACCGCGTTC 30 TAATACGACTCACTATAGGCGTAGCCTGATGAGTT CA CACTGGCTGCACCCACCACCGCGTTCCACGAAACG TGGTGAAAGCCACGTAGCTGCGCC 26 CATCCACGGTGACGCTAATCCCACGTTC 31 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA GA TCCACGGTGACGCTAATCCCACGTTCGACGAAACG TGGTGAAAGCCACGTAGCTGCGCC 27 ACAATGCAGATGCGCCCACCACGGATCA 32 TAATACGACTCACTATAGGCGTAGCCTGATGAGAC CT AATGCAGATGCGCCCACCACGGATCACTCGAAACG TGGTGAAAGCCACGTAGCTGCGCC 28 CAACCAAGCACGCTGCATCACGTTTCAT 33 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA CG ACCAAGCACGCTGCATCACGTTTCATCGCGAAACG TGGTGAAAGCCACGTAGCTGCGCC 29 CTCACAGCCCGAAACACATCGCCACGTT 34 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT CA CACAGCCCGAAACACATCGCCACGTTCACGAAACG TGGTGAAAGCCACGTAGCTGCGCC Fish 35 CTCAATACTACGTCAATTCACAGATGAT 41 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT AGACACCACGGA CAATACTACGTCAATTCACAGATGATAGACACCAC GGACGAAACGTGGTGAAAGCCACGTAGCTGCGCC 36 TCCAACACCACGTAACGTACACTGCATG 42 TAATACGACTCACTATAGGCGTAGCCTGATGAGTC TGATTGGTGCAA CAACACCACGTAACGTACACTGCATGTGATTGGTG CAACGAAACGTGGTGAAAGCCACGTAGCTGCGCC 37 TGGCGCCGACTGATCAACTAGACATCAC 43 TAATACGACTCACTATAGGCGTAGCCTGATGAGTG GTTAGCATTCCG GCGCCGACTGATCAACTAGACATCACGTTAGCATT CCGCGAAACGTGGTGAAAGCCACGTAGCTGCGCC 38 CCAGCAACCAGGTTACCTCCCATCACGC 44 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC TTCGTCTCAGGA AGCAACCAGGTTACCTCCCATCACGCTTCGTCTCA GGACGAAACGTGGTGAAAGCCACGTAGCTGCGCC 39 CTGACACCACAAACGATTATGACCACGT 45 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT TATCGTACATAG GACACCACAAACGATTATGACCACGTTATCGTACA TAGCGAAACGTGGTGAAAGCCACGTAGCTGCGCC 40 TAGGTCAAGTGCGCTAAAACACACCGCG 46 TAATACGACTCACTATAGGCGTAGCCTGATGAGTA TTAGTTCACCAA GGTCAAGTGCGCTAAAACACACCGCGTTAGTTCAC CAACGAAACGTGGTGAAAGCCACGTAGCTGCGCC Egg 47 GGCCACCTCACTGTGTTTTGTTGCACAA 53 TAATACGACTCACTATAGGCGTAGCCTGATGAGGC CATAATATGATGACGTGC CACCTCACTGTGTTTTGTTGCACAACATAATATGA TGACGTGCCGAAACGTGGTGAAAGCCACGTAGCTG CGCC 48 GCGTTCCCCACCGTTGCCCACGCTTAAC 54 TAATACGACTCACTATAGGCGTAGCCTGATGAGGC TGGACAAAGATGGGCCC GTTCCCCACCGTTGCCCACGCTTAACTGGACAAAG ATGGGCCCCGAAACGTGGTGAAAGCCACGTAGCTG CGCC 49 TCTGTGCACATCACTCGACCTCTACGGC 55 TAATACGACTCACTATAGGCGTAGCCTGATGAGTC TGTATTGATCCTGCATA TGTGCACATCACTCGACCTCTACGGCTGTATTGAT CCTGCATACGAAACGTGGTGAAAGCCACGTAGCTG CGCC 50 CGTCCAACGTTCGATCAGAACCGCGTTC 56 TAATACGACTCACTATAGGCGTAGCCTGATGAGCG AGGCTGATGATTGTACG TCCAACGTTCGATCAGAACCGCGTTCAGGCTGATG ATTGTACGCGAAACGTGGTGAAAGCCACGTAGCTG CGCC 51 CATCAGTGCGTTCTGCCTTTGCAACCAC 57 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA ACAACACACCGTATGAG TCAGTGCGTTCTGCCTTTGCAACCACACAACACAC CGTATGAGCGAAACGTGGTGAAAGCCACGTAGCTG CGCC 52 CCAACTGTGCACACTGTTCGCTTATCGA 58 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC GCTGTGTACCTCCATAG AACTGTGCACACTGTTCGCTTATCGAGCTGTGTAC CTCCATAGCGAAACGTGGTGAAAGCCACGTAGCTG CGCC Gluten 59 CTTGGTCACCTTTCCTGACATTAACACA 65 TAATACGACTCACTATAGGCGTAGCCTGATGAGCT GG TGGTCACCTTTCCTGACATTAACACAGGCGAAACG TGGTGAAAGCCACGTAGCTGCGCC 60 TTTTCCCGATACGGCTACGAATTGCGAC 66 TAATACGACTCACTATAGGCGTAGCCTGATGAGTT AA TTCCCGATACGGCTACGAATTGCGACAACGAAACG TGGTGAAAGCCACGTAGCTGCGCC 61 GCACCAATTTTACCGATTTTGGTGGACA 67 TAATACGACTCACTATAGGCGTAGCCTGATGAGGC GC ACCAATTTTACCGATTTTGGTGGACAGCCGAAACG TGGTGAAAGCCACGTAGCTGCGCC 62 CGTACAACCCACCACCGTTGTCCACAAA 68 TAATACGACTCACTATAGGCGTAGCCTGATGAGCG TG TACAACCCACCACCGTTGTCCACAAATGCGAAACG TGGTGAAAGCCACGTAGCTGCGCC 63 TGCGTCAACGGCCGTCCCGAAACGTGAA 69 TAATACGACTCACTATAGGCGTAGCCTGATGAGTG TA CGTCAACGGCCGTCCCGAAACGTGAATACGAAACG TGGTGAAAGCCACGTAGCTGCGCC 64 GTTACCCCGAAACGGCCCTAACTGCATC 70 TAATACGACTCACTATAGGCGTAGCCTGATGAGGT AG TACCCCGAAACGGCCCTAACTGCATCAGCGAAACG TGGTGAAAGCCACGTAGCTGCGCC Soy 71 CCGCATCACCACCCAAACCACCGTT 76 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC GCATCACCACCCAAACCACCGTTCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 72 CCTGCTCCATCCGCGCCAGCCTCAC 77 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC TGCTCCATCCGCGCCAGCCTCACCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 73 CCAATCTCCTGCCCACGCCGTTCCA 78 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC AATCTCCTGCCCACGCCGTTCCACGAAACGTGGTG AAAGCCACGTAGCTGCGCC 74 CCAATCAAGGACCGCCTTCACCGCT 79 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC AATCAAGGACCGCCTTCACCGCTCGAAACGTGGTG GAAAGCCACGTAGCTGCGCC 75 ACTCTCGCATCACCAGCCAACTCAC 80 TAATACGACTCACTATAGGCGTAGCCTGATGAGAC TCTCGCATCACCAGCCAACTCACCGAAACGTGGTG AAAGCCACGTAGCTGCGCC Crustacean 81 CGGTACTCAGATTACAGAGTGACAT 86 TAATACGACTCACTATAGGCGTAGCCTGATGAGCG GTACTCAGATTACAGAGTGACATCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 82 AGACACCACGGATCCGAACTGGAG 87 TAATACGACTCACTATAGGCGTAGCCTGATGAGAG ACACCACGGATCCGAACTGGAGCGAAACGTGGTGA AAGCCACGTAGCTGCGCC 83 CCTCGCAAGATTGCATACGTTAGAA 88 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC TCGCAAGATTGCATACGTTAGAACGAAACGTGGTG AAAGCCACGTAGCTGCGCC 84 CACGTAGGAAACGACCTCTACGGAG 89 TAATACGACTCACTATAGGCGTAGCCTGATGAGCA CGTAGGAAACGACCTCTACGGAGCGAAACGTGGTG AAAGCCACGTAGCTGCGCC 85 CCCGAAACCACCACCGTTGTCCAATA 90 TAATACGACTCACTATAGGCGTAGCCTGATGAGCC CGAAACCACCACCGTTGTCCAATACGAAACGTGGT GAAAGCCACGTAGCTGCGCC

In some embodiments, signaling polynucleotides of the present invention may be generated by modifying the original allergen binding aptamers disclosed in the literature. The parent sequence of each aptamer against a specific allergen is modified to comprise the shortest sequence without changing the binding specificity and affinity of the aptamer. Some exemplary signaling polynucleotides modified from known parent sequences are listed in Table 2.

TABLE 2 SPNs originated from literature sequences Allergen Description SEQ ID NO. Sequence (5′-3′) Gluten GLI4- 91 CCAGTCTCCCGTTTACCGCGCCTACACATGT aptamersequence CTGAATGCC GLI4- 92 CTAGGCGAAATATAGCTACAACTGTCTGAAG aptamersequence GCACCCAAT Egg Aptamersequence 93 ATCTACGAATTCATCAGGGCTAAAGAGTGCA GAGTTACTTAG Aptamer 94 GCAGCTAAGCAGGCGGCTCACAAAACCATTC sequence GCATGCGGC Ellington apatmer 95 GGUUGUGAAGAUUGGGAGCGUCGUGGCUAC and Cox sequence ARAH1-aptamer 96 TCGCACATTCCGCTTCTACCGGGGGGGTCGA sequence GCTGAGTGGATGCGAATCTGTGGGTGGGCCG TAAGTCCGTGTGTGCGAA

In some embodiments, aptamer sequences that specific bind to peanut allergen and tree nut allergen were selected through SELEX and top 100 sequences with high relative abundance were selected from each SELEX selection. Their unique sequences and full sequences including the primer sequences are listed in Table 3 (peanut) and Table 4 (tree nut). Complementary sequences specific to an aptamer may be synthesized and screened for the best binding specificity to its corresponding SPN and to the solid support.

TABLE 3 Aptamers against peanut antigen SEQ ID NO. Unique Sequence (5′-3′) SEQ ID NO. Full sequence including primers (5′-3′)  97 GGCCTGCGATGGATGTGTGCGTG 297 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATTAGC GTGCGTGTATTAGCTTGACTAGTACATGACCACTTGA  98 GTACGCGCTCTGGATGTGGTTTG 298 TAGGGAAGAGAAGGACATATGATGTACGCGCTCTGGATG TTAGTCT TGGTTTGTTAGTCTTTGACTAGTACATGACCACTTGA  99 GGCCGGCGATGGATGTGGTTGTG 299 TAGGGAAGAGAAGGACATATGATGGCCGGCGATGGATGT CTTGTTT GGTTGTGCTTGTTTTTGACTAGTACATGACCACTTGA 100 GTGCGACCGACCCTATCAGGTGC 300 TAGGGAAGAGAAGGACATATGATGTGCGACCGACCCTAT TCATGTA CAGGTGCTCATGTATTGACTAGTACATGACCACTTGA 101 GGCCGCGTCTGGATGTGGTTTTG 301 TAGGGAAGAGAAGGACATATGATGGCCGCGTCTGGATGT TCGCGTC GGTTTTGTCGCGTCTTGACTAGTACATGACCACTTGA 102 GTCCGACGATGGATGTGGATGTA 302 TAGGGAAGAGAAGGACATATGATGTCCGACGATGGATGT TTGGTCT GGATGTATTGGTCTTTGACTAGTACATGACCACTTGA 103 GGCCTGCGATGGATGTGGGCTAG 303 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATGGGC GGGCTAGTATGGGCTTGACTAGTACATGACCACTTGA 104 GTTCCGCCGATGGATGTGGGTGT 304 TAGGGAAGAGAAGGACATATGATGTTCCGCCGATGGATG AGTTGTC TGGGTGTAGTTGTCTTGACTAGTACATGACCACTTGA 105 GGCATTCGATGGATGGGGTGGTG 305 TAGGGAAGAGAAGGACATATGATGGCATTCGATGGATGG TTAGTCT GGTGGTGTTAGTCTTTGACTAGTACATGACCACTTGA 106 GTCCGCAGCTGGATGGGGGAGTG 306 TAGGGAAGAGAAGGACATATGATGTCCGCAGCTGGATGG TCTGGTT GGGAGTGTCTGGTTTTGACTAGTACATGACCACTTGA 107 GTCAGTCGATGGATGTGGGTTGT 307 TAGGGAAGAGAAGGACATATGATGTCAGTCGATGGATGT GCTCGTC GGGTTGTGCTCGTCTTGACTAGTACATGACCACTTGA 108 GTACGACGCGGACCTTCAAGTAG 308 TAGGGAAGAGAAGGACATATGATGTACGACGCGGACCTT GCGTGTA CAAGTAGGCGTGTATTGACTAGTACATGACCACTTGA 109 GGCCTCGAAGCCCTTCAAGCGGT 309 TAGGGAAGAGAAGGACATATGATGGCCTCGAAGCCCTTC TCATGGA AAGCGGTTCATGGATTGACTAGTACATGACCACTTGA 110 GGCCGATCTGGATGGGGGCTCGG 310 TAGGGAAGAGAAGGACATATGATGGCCGATCTGGATGGG GCGAGTC GGCTCGGGCGAGTCTTGACTAGTACATGACCACTTGA 111 GGCCTGCGATGGATGAGGTGCTG 311 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGA CACTAGT GGTGCTGCACTAGTTTGACTAGTACATGACCACTTGA 112 GTACGCGCTCTGGATGTGGTTGG 312 TAGGGAAGAGAAGGACATATGATGTACGCGCTCTGGATG TTAGTCT TGGTTGGTTAGTCTTTGACTAGTACATGACCACTTGA 113 GGCCGCCGATGGATGTTGGCATT 313 TAGGGAAGAGAAGGACATATGATGGCCGCCGATGGATGT GCTGGTC TGGCATTGCTGGTCTTGACTAGTACATGACCACTTGA 114 GGCCGATCTGGATGGGGTATGTG 314 TAGGGAAGAGAAGGACATATGATGGCCGATCTGGATGGG TCTAGGC GTATGTGTCTAGGCTTGACTAGTACATGACCACTTGA 115 GTCCGTCGATGGATGGGGTTGGG 315 TAGGGAAGAGAAGGACATATGATGTCCGTCGATGGATGG TTCAGTC GGTTGGGTTCAGTCTTGACTAGTACATGACCACTTGA 116 GTGCTTGGATCCCTATCAGGTGG 316 TAGGGAAGAGAAGGACATATGATGTGCTTGGATCCCTAT ACGTGTA CAGGTGGACGTGTATTGACTAGTACATGACCACTTGA 117 GTCGTTCGATGGATGTGTGCTGT 317 TAGGGAAGAGAAGGACATATGATGTCGTTCGATGGATGT ATGAGTC GTGCTGTATGAGTCTTGACTAGTACATGACCACTTGA 118 GTCCGACGATGGGTGGGGGAATG 318 TAGGGAAGAGAAGGACATATGATGTCCGACGATGGGTGG CGACGGC GGGAATGCGACGGCTTGACTAGTACATGACCACTTGA 119 GTGCGCCGATGGGTGTGTGTCGT 319 TAGGGAAGAGAAGGACATATGATGTGCGCCGATGGGTGT GGCTGGT GTGTCGTGGCTGGTTTGACTAGTACATGACCACTTGA 120 GTCCTGATCTGGGTGTGGGGGTG 320 TAGGGAAGAGAAGGACATATGATGTCCTGATCTGGGTGT TGCAGGC GGGGGTGTGCAGGCTTGACTAGTACATGACCACTTGA 121 GGCCTGACTGGGTGTGGGTAGTT 321 TAGGGAAGAGAAGGACATATGATGGCCTGACTGGGTGTG ACTTGGC GGTAGTTACTTGGCTTGACTAGTACATGACCACTTGA 122 GGACGCATCGCCCCTTCGAGTGG 322 TAGGGAAGAGAAGGACATATGATGGACGCATCGCCCCTT ACAGGTA CGAGTGGACAGGTATTGACTAGTACATGACCACTTGA 123 GGCCTGACTGGGTGTGGTTAGGA 323 TAGGGAAGAGAAGGACATATGATGGCCTGACTGGGTGTG ACGCGTC GTTAGGAACGCGTCTTGACTAGTACATGACCACTTGA 124 GTCATGCGATGGATGGGGGCTGG 324 TAGGGAAGAGAAGGACATATGATGTCATGCGATGGATGG CAGTCGT GGGCTGGCAGTCGTTTGACTAGTACATGACCACTTGA 125 AATGTGGCGGGATCTGGATGTGT 325 TAGGGAAGAGAAGGACATATGATAATGTGGCGGGATCTG GCATGTA GATGTGTGCATGTATTGACTAGTACATGACCACTTGA 126 GGCCTGGTCTGGATGGGGGCGGG 326 TAGGGAAGAGAAGGACATATGATGGCCTGGTCTGGATGG TATAGGC GGGCGGGTATAGGCTTGACTAGTACATGACCACTTGA 127 GGCCTGGGATGGATGTGGTGTAT 327 TAGGGAAGAGAAGGACATATGATGGCCTGGGATGGATGT TAGGCTG GGTGTATTAGGCTGTTGACTAGTACATGACCACTTGA 128 GCCCGACTCTGGATGGGGGAATG 328 TAGGGAAGAGAAGGACATATGATGCCCGACTCTGGATGG CGCAGTC GGGAATGCGCAGTCTTGACTAGTACATGACCACTTGA 129 GTCGTGCTCTGGGTGGGGTTGTG 329 TAGGGAAGAGAAGGACATATGATGTCGTGCTCTGGGTGG TAGTAGT GGTTGTGTAGTAGTTTGACTAGTACATGACCACTTGA 130 GTCATTCGCTGGATGTGTTGATG 330 TAGGGAAGAGAAGGACATATGATGTCATTCGCTGGATGT TCTGGTC GTTGATGTCTGGTCTTGACTAGTACATGACCACTTGA 131 GGCCGGCGATGGATGTGTATGTG 331 TAGGGAAGAGAAGGACATATGATGGCCGGCGATGGATGT GTAGTCG GTATGTGGTAGTCGTTGACTAGTACATGACCACTTGA 132 GGACGCGGCTGGATGGGGGCTTG 332 TAGGGAAGAGAAGGACATATGATGGACGCGGCTGGATGG CACTGTC GGGCTTGCACTGTCTTGACTAGTACATGACCACTTGA 133 GGCCGGCGATGGATGTGTGCGTG 333 TAGGGAAGAGAAGGACATATGATGGCCGGCGATGGATGT TATTAGC GTGCGTGTATTAGCTTGACTAGTACATGACCACTTGA 134 GGCCGCCGATGGGTGTGGAGGTG 334 TAGGGAAGAGAAGGACATATGATGGCCGCCGATGGGTGT TACTTGT GGAGGTGTACTTGTTTGACTAGTACATGACCACTTGA 135 GGCCTGCGATGGATGTGGTTGTG 335 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT CTTGTTT GGTTGTGCTTGTTTTTGACTAGTACATGACCACTTGA 136 GGCCGACGATGGCGTAGCGTCTG 336 TAGGGAAGAGAAGGACATATGATGGCCGACGATGGCGTA TACTGTT GCGTCTGTACTGTTTTGACTAGTACATGACCACTTGA 137 GGCCGTGTCTGGGTGGGGGTATG 337 TAGGGAAGAGAAGGACATATGATGGCCGTGTCTGGGTGG CACTGTC GGGTATGCACTGTCTTGACTAGTACATGACCACTTGA 138 GGCCGGCGATGGATGTGAAATGG 338 TAGGGAAGAGAAGGACATATGATGGCCGGCGATGGATGT CTTGTCT GAAATGGCTTGTCTTTGACTAGTACATGACCACTTGA 139 GGCCGCGTCTGGGTGTTGGTTGT 339 TAGGGAAGAGAAGGACATATGATGGCCGCGTCTGGGTGT GTTAGGC TGGTTGTGTTAGGCTTGACTAGTACATGACCACTTGA 140 GGACAGCGATGGATGTGGAAATG 340 TAGGGAAGAGAAGGACATATGATGGACAGCGATGGATGT CGACGTC GGAAATGCGACGTCTTGACTAGTACATGACCACTTGA 141 GGACTGCGCGTGACCTATCAATG 341 TAGGGAAGAGAAGGACATATGATGGACTGCGCGTGACCT GCATGTA ATCAATGGCATGTATTGACTAGTACATGACCACTTGA 142 GGCCAGCTCTGGATGAGGTCTGT 342 TAGGGAAGAGAAGGACATATGATGGCCAGCTCTGGATGA GCGAGGC GGTCTGTGCGAGGCTTGACTAGTACATGACCACTTGA 143 GTCCGACCGCACCCTTCGAGGGG 343 TAGGGAAGAGAAGGACATATGATGTCCGACCGCACCCTT ACATGGA CGAGGGGACATGGATTGACTAGTACATGACCACTTGA 144 GGCCAATGCGCCCCTTCATGTTG 344 TAGGGAAGAGAAGGACATATGATGGCCAATGCGCCCCTT TCGTGTA CATGTTGTCGTGTATTGACTAGTACATGACCACTTGA 145 GGCCGGCTATACCCTACACGTGA 345 TAGGGAAGAGAAGGACATATGATGGCCGGCTATACCCTA TCAGGTA CACGTGATCAGGTATTGACTAGTACATGACCACTTGA 146 GTGCGCACGATGGATGTGGATGG 346 TAGGGAAGAGAAGGACATATGATGTGCGCACGATGGATG CCAGTCT TGGATGGCCAGTCTTTGACTAGTACATGACCACTTGA 147 GGCATGCGATGGATGGGGGCTGG 347 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGG GGCAGTC GGGCTGGGGCAGTCTTGACTAGTACATGACCACTTGA 148 GTCATGCGCTGGATGTGGGTTGT 348 TAGGGAAGAGAAGGACATATGATGTCATGCGCTGGATGT TATAGGC GGGTTGTTATAGGCTTGACTAGTACATGACCACTTGA 149 GTGCGCCTCTGGATGGGGTTTGT 349 TAGGGAAGAGAAGGACATATGATGTGCGCCTCTGGATGG CGACGGC GGTTTGTCGACGGCTTGACTAGTACATGACCACTTGA 150 GGCCAGCTCTGGATGTGGCATTG 350 TAGGGAAGAGAAGGACATATGATGGCCAGCTCTGGATGT TCTGGTC GGCATTGTCTGGTCTTGACTAGTACATGACCACTTGA 151 GGCCTGAGCTGGCATTGCGCTGG 351 TAGGGAAGAGAAGGACATATGATGGCCTGAGCTGGCATT ACATGTA GCGCTGGACATGTATTGACTAGTACATGACCACTTGA 152 GGCCGCCGATGGGTGTGGGATCG 352 TAGGGAAGAGAAGGACATATGATGGCCGCCGATGGGTGT TGCGGGC GGGATCGTGCGGGCTTGACTAGTACATGACCACTTGA 153 GGCCGACGCTGGGTGGGGGCGTT 353 TAGGGAAGAGAAGGACATATGATGGCCGACGCTGGGTGG GACTACGT GGGCGTTGACTAGTTTGACTAGTACATGACCACTTGA 154 GGACTACGCTGGATGGGGACATT 354 TAGGGAAGAGAAGGACATATGATGGACTACGCTGGATGG GCTAGTT GGACATTGCTAGTTTTGACTAGTACATGACCACTTGA 155 GGCATGCGATGGGTGTGTTCTGG 355 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGGTGT CGACGGC GTTCTGGCGACGGCTTGACTAGTACATGACCACTTGA 156 GGACTACGCTGGATGTGGGTTGG 356 TAGGGAAGAGAAGGACATATGATGGACTACGCTGGATGT GGTAGTC GGGTTGGGGTAGTCTTGACTAGTACATGACCACTTGA 157 GGCCGAGCTTACCTGTCAAGTGC 357 TAGGGAAGAGAAGGACATATGATGGCCGAGCTTACCTGT GAGTGTA CAAGTGCGAGTGTATTGACTAGTACATGACCACTTGA 158 GTGCTTCGATGGATGTGGGCGTT 358 TAGGGAAGAGAAGGACATATGATGTGCTTCGATGGATGT GCAAGTC GGGCGTTGCAAGTCTTGACTAGTACATGACCACTTGA 159 GTCCGCGGCTGGGTGTGGGAAGT 359 TAGGGAAGAGAAGGACATATGATGTCCGCGGCTGGGTGT ACTCGGC GGGAAGTACTCGGCTTGACTAGTACATGACCACTTGA 160 GTCCGCGCGATGGATGAGGACGT 360 TAGGGAAGAGAAGGACATATGATGTCCGCGCGATGGATG GAGCTAG AGGACGTGAGCTAGTTGACTAGTACATGACCACTTGA 161 GGCCGAGTCGTCACTTCAATTGG 361 TAGGGAAGAGAAGGACATATGATGGCCGAGTCGTCACTT GCGTGGA CAATTGGGCGTGGATTGACTAGTACATGACCACTTGA 162 GTCGGTCGGAGGGATGGTCTCGT 362 TAGGGAAGAGAAGGACATATGATGTCGGTCGGAGGGATG TGACGGC GTCTCGTTGACGGCTTGACTAGTACATGACCACTTGA 163 GGCCACACGCTGCCCTAAAGTGT 363 TAGGGAAGAGAAGGACATATGATGGCCACACGCTGCCCT TCGTGTA AAAGTGTTCGTGTATTGACTAGTACATGACCACTTGA 164 GGCCTGCGATGGATGTGTGCGTG 364 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATTAGT GTGCGTGTATTAGTTTGACTAGTACATGACCACTTGA 165 GTGCGCTGTCTTGCCTACAAGTG 365 TAGGGAAGAGAAGGACATATGATGTGCGCTGTCTTGCCT TCGTGTA ACAAGTGTCGTGTATTGACTAGTACATGACCACTTGA 166 GGCCGGAACTGGATGGGGGCATT 366 TAGGGAAGAGAAGGACATATGATGGCCGAACTGGATGGG ACTGCGGC GGCATTACTGCGGCTTGACTAGTACATGACCACTTGA 167 GGCCGAGCTGGATGGGGTATTGG 367 TAGGGAAGAGAAGGACATATGATGGCCGAGCTGGATGGG ATCTAGT GTATTGGATCTAGTTTGACTAGTACATGACCACTTGA 168 TGGCCGCACTCTGGGTGTGGTGG 368 TAGGGAAGAGAAGGACATATGATTGGCCGCACTCTGGGT ACTTGGC GTGGTGGACTTGGCTTGACTAGTACATGACCACTTGA 169 GGCCGGTCTGGATGGGGGCGTAC 369 TAGGGAAGAGAAGGACATATGATGGCCGGTCTGGATGGG GTCGTCG GGCGTACGTCGTCGTTGACTAGTACATGACCACTTGA 170 GGCCTGCTATGGGTGGGGGCTCG 370 TAGGGAAGAGAAGGACATATGATGGCCTGCTATGGGTGG TACTGGC GGGCTCGTACTGGCTTGACTAGTACATGACCACTTGA 171 GTACGCCCGATGGATGTGGATTG 371 TAGGGAAGAGAAGGACATATGATGTACGCCCGATGGATG TACTGTT TGGATTGTACTGTTTTGACTAGTACATGACCACTTGA 172 GGCCTGCGATGGATGTGGGCCAG 372 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TACGCGC GGGCCAGTACGCGCTTGACTAGTACATGACCACTTGA 173 GACCTGCGATGGGTGTGGCTCTG 373 TAGGGAAGAGAAGGACATATGATGACCTGCGATGGGTGT TCAGTCT GGCTCTGTCAGTCTTTGACTAGTACATGACCACTTGA 174 GTCCGAACTGGATGTGGTATTGG 374 TAGGGAAGAGAAGGACATATGATGTCCGAACTGGATGTG CCTGTCT GTATTGGCCTGTCTTTGACTAGTACATGACCACTTGA 175 GTTCTTGTCTGGATGGGGTTGAT 375 TAGGGAAGAGAAGGACATATGATGTTCTTGTCTGGATGG GTCGGTC GGTTGATGTCGGTCTTGACTAGTACATGACCACTTGA 176 GTACTCGATGGGTGTGGGTAGGC 376 TAGGGAAGAGAAGGACATATGATGTACTCGATGGGTGTG GCGAGTC GGTAGGCGCGAGTCTTGACTAGTACATGACCACTTGA 177 GTCCTCGATGGGTGTGAGATATG 377 TAGGGAAGAGAAGGACATATGATGTCCTCGATGGGTGTG TGCTAGC AGATATGTGCTAGCTTGACTAGTACATGACCACTTGA 178 GGCCGTGCTCTGGGTGTGGGCCT 378 TAGGGAAGAGAAGGACATATGATGGCCGTGCTCTGGGTG GCTGGGC TGGGCCTGCTGGGCTTGACTAGTACATGACCACTTGA 179 GTTCGTATCTGGGGTGTGGTGTG 379 TAGGGAAGAGAAGGACATATGATGTTCGTATCTGGGTGT TCTGGGCT GGTGTGTCTGGGCTTTGACTAGTACATGACCACTTGA 180 GGCCGAGTCTGGATGTGTGTCGT 380 TAGGGAAGAGAAGGACATATGATGGCCGAGTCTGGATGT ACGTATC GTGTCGTACGTATCTTGACTAGTACATGACCACTTGA 181 GGCGTTCACTGGGTGTGGATGTG 381 TAGGGAAGAGAAGGACATATGATGGCGTTCACTGGGTGT TGCGGTC GGATGTGTGCGGTCTTGACTAGTACATGACCACTTGA 182 GTCATGCGCTGGGTGTGGCCTGT 382 TAGGGAAGAGAAGGACATATGATGTCATGCGCTGGGTGT TGTAGGC GGCCTGTTGTAGGCTTGACTAGTACATGACCACTTGA 183 GCTCCGTACGATGGCTGTGCTGG 383 TAGGGAAGAGAAGGACATATGATGCTCCGTACGATGGCT TGATGTA GTGCTGGTGATGTATTGACTAGTACATGACCACTTGA 184 GGACTGCGATGGGTGGGGTTATG 384 TAGGGAAGAGAAGGACATATGATGGACTGCGATGGGTGG TGCCAGC GGTTATGTGCCAGCTTGACTAGTACATGACCACTTGA 185 GTGCGATCGTACCTATCAATGGT 385 TAGGGAAGAGAAGGACATATGATGTGCGATCGTACCTAT CATCGTA CAATGGTCATCGTATTGACTAGTACATGACCACTTGA 186 GTTCGTCGAATGGATGTGAGCAT 386 TAGGGAAGAGAAGGACATATGATGTTCGTCGAATGGATG GTCTGTC TGAGCATGTCTGTCTTGACTAGTACATGACCACTTGA 187 GGCCGTACGATGGATGTGGGATG 387 TAGGGAAGAGAAGGACATATGATGGCCGTACGATGGATG GTCTAGC TGGGATGGTCTAGCTTGACTAGTACATGACCACTTGA 188 GTCATTAACTGGATGTGGGACTG 388 TAGGGAAGAGAAGGACATATGATGTCATTAACTGGATGT TCGGTCT GGGACTGTCGGTCTTTGACTAGTACATGACCACTTGA 189 GGACGATCTGGGTGTGGACAGGG 389 TAGGGAAGAGAAGGACATATGATGGACGATCTGGGTGTG ATGAGGC GACAGGGATGAGGCTTGACTAGTACATGACCACTTGA 190 GGCATGCGATGGATGTGGTGTAC 390 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGT CCAGTCC GGTGTACCCAGTCCTTGACTAGTACATGACCACTTGA 191 GGCCGCGATGGATGTGGAAAGGT 391 TAGGGAAGAGAAGGACATATGATGGCCGCGATGGATGTG CTAGTCA GAAAGGTCTAGTCATTGACTAGTACATGACCACTTGA 192 GGCCGACCTGGATGTGAGCATGC 392 TAGGGAAGAGAAGGACATATGATGGCCGACCTGGATGTG ATCTAGT AGCATGCATCTAGTTTGACTAGTACATGACCACTTGA 193 GTACGAGCGGACCGATCAAGTGC 393 TAGGGAAGAGAAGGACATATGATGTACGAGCGGACCGAT GTCTGTA CAAGTGCGTCTGTATTGACTAGTACATGACCACTTGA 194 GTACTGCACTGCCCTACACGTGG 394 TAGGGAAGAGAAGGACATATGATGTACTGCACTGCCCTA GAATGGA CACGTGGGAATGGATTGACTAGTACATGACCACTTGA 195 GTCATTCGATGGATGTGGCGTGT 395 TAGGGAAGAGAAGGACATATGATGTCATTCGATGGATGT GCGTCAT GGCGTGTGCGTCATTTGACTAGTACATGACCACTTGA 196 GGCGTACGATGGATTGCGTTGTG 396 TAGGGAAGAGAAGGACATATGATGGCGTACGATGGATGT TCTGTC GCGTTGTGTCTGTCTTGACTAGTACATGACCACTTGA 197 GGCCTGCGATGGATGTGTGCGTG 397 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATTAGC GTGCGTGTATTAGCTTGACTAGTACATGACCACTTGA 198 GTCATTCCGCATCCTACACGTGG 398 TAGGGAAGAGAAGGACATATGATGTCATTCCGCATCCTA GCACGTA CACGTGGGCACGTATTGACTAGTACATGACCACTTGA 199 GGCCAATGCGCCCCTTCATGTTG 399 TAGGGAAGAGAAGGACATATGATGGCCAATGCGCCCCTT TCGTGTA CATGTTGTCGTGTATTGACTAGTACATGACCACTTGA 200 GGCCTGCGATGGATAGGTGCTGC 400 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGA ACTAGT GGTGCTGCACTAGTTTGACTAGTACATGACCACTTGA 201 GTCAGTCGATGGATGTGGGTTGT 401 TAGGGAAGAGAAGGACATATGATGTCAGTCGATGGATGT GCTCGTC GGGTTGTGCTCGTCTTGACTAGTACATGACCACTTGA 202 GTCGTGACTGGCTAGCTGGACAT 402 TAGGGAAGAGAAGGACATATGATGTCGTGACTGGCTAGCT GCACTGC GGACATGCACTGCTTGACTAGTACATGACCACTTGA 203 GGCCTGCGATGGATGTGGGCTAG 403 TAGTGGAAGAGAAGGACATATGATGGCCTGCGATGGATG TATGGGC TGGGCTAGTATGGGCTTGACTAGTACATGACCACTTGA 204 GTGCATCGATGGCGTATGCTGGT 404 TAGGGAAGAGAAGGACATATGATGTGCATCGATGGCGTAT GATGTGC GCTGGTGATGTGCTTGACTAGTACATGACCACTTGA 205 GCGACAGCGACATACGATCTGCT 405 TAGGGAAGAGAAGGACATATGATGCGACAGCGACATACG CTGCGTC ATCTGCTCTGCGTCTTGACTAGTACATGACCACTTGA 206 GTCATGCCATCCCTTCGAGTGTG 406 TAGGGAAGAGAAGGACATATGATGTCATGCCATCCCTTC ACAGGTA GAGTGTGACAGGTATTGACTAGTACATGACCACTTGA 207 GGCCTGACTGGGTGTGGTTAGGA 407 TAGGGAAGAGAAGGACATATGATGGCCTGACTGGGTGTG ACGCGTC GTTAGGAACGCGTCTTGACTAGTACATGACCACTTGA 208 GTGCGCACGATGGATGTGGATGG 408 TAGGGAAGAGAAGGACATATGATGTGCGCACGATGGATG CCAGTCT TGGATGGCCAGTCTTTGACTAGTACATGACCACTTGA 209 GTGCGCCGATGGGTGTGTGTCGT 409 TAGGGAAGAGAAGGACATATGATGTGCGCCGATGGGTGT GGCTGGT GTGTCGTGGCTGGTTTGACTAGTACATGACCACTTGA 210 GGCATGCGATGGATGTGGTGTAC 410 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGT CCAGTCC GGTGTACCCAGTCCTTGACTAGTACATGACCACTTGA 211 CCATATGGCAGTGCGATGGCTTC 411 TAGGGAAGAGAAGGACATATGATCCATATGGCAGTGCGA GCTGGTC TGGCTTCGCTGGTCTTGACTAGTACATGACCACTTGA 212 GCTCCGTACGATGGCTGTGCTGG 412 TAGGGAAGAGAAGGACATATGATGCTCCGTACGATGGCT TGATGTA GTGCTGGTGATGTATTGACTAGTACATGACCACTTGA 213 GTGCGACCGACCCTATCAGGTGC 413 TAGGGAAGAGAAGGACATATGATGTGCGACCGACCCTAT TCATGTA CAGGTGCTCATGTATTGACTAGTACATGACCACTTGA 214 GTTCCGCCGATGGATGTGGGTGT 414 TAGGGAAGAGAAGGACATATGATGTTCCGCCGATGGATG AGTTGTC TGGGTGTAGTTGTCTTGACTAGTACATGACCACTTGA 215 GTACTGCACTGCCCTACACGTGG 415 TAGGGAAGAGAAGGACATATGATGTACTGCACTGCCCTA GAATGGA CACGTGGGAATGGATTGACTAGTACATGACCACTTGA 216 CGCACCGTCGATACGTCATGCAC 416 TAGGGAAGAGAAGGACATATGATCGCACCGTCGATACGTC GCTGACA ATGCACGCTGACATTGACTAGTACATGACCACTTGA 217 GTACGCACGATGAGCGCCAAGTG 417 TAGGGAAGAGAAGGACATATGATGTACGCACGATGAGCG ACATGGA CCAAGTGACATGGATTGACTAGTACATGACCACTTGA 218 GTCGGTCGGAGGGATGGTCTCGT 418 TAGGGAAGAGAAGGACATATGATGTCGGTCGGAGGGATG TGACGGC GTCTCGTTGACGGCTTGACTAGTACATGACCACTTGA 219 GGCATGCGATGAACGAGGCATGA 419 TAGGGAAGAGAAGGACATATGATGGCATGCGATGAACGA TGCGTCA GGCATGATGCGTCATTGACTAGTACATGACCACTTGA 220 GGCGTACGATGGATGTGCGTTGT 420 TAGGGAAGAGAAGGACATATGATGGCGTACGATGGATGT GTCTGTC GCGTTGTGTCTGTCTTGACTAGTACATGACCACTTGA 221 GTCACTGTGCCTGACCGTCAAGT 421 TAGGGAAGAGAAGGACATATGATGTCACTGTGCCTGACC TGCGGCA GTCAAGTTGCGGCATTGACTAGTACATGACCACTTGA 222 GGACTGCGCGTGACCTATCAATG 422 TAGGGAAGAGAAGGACATATGATGGACTGCGCGTGACCT GCATGTA ATCAATGGCATGTATTGACTAGTACATGACCACTTGA 223 GGCCTGAGCTGGCATTGCGCTGG 423 TAGGGAAGAGAAGGACATATGATGGCCTGAGCTGGCATT ACATGTA GCGCTGGACATGTATTGACTAGTACATGACCACTTGA 224 GCATTGGACGATCGTGCCCTACA 424 TAGGGAAGAGAAGGACATATGATGCATTGGACGATCGTG CGTGGGC CCCTACACGTGGGCTTGACTAGTACATGACCACTTGA 225 GGACGCATCGCCCCTTCGAGTGG 425 TAGGGAAGAGAAGGACATATGATGGACGCATCGCCCCTT ACAGGTA CGAGTGGACACGGTATTGACTAGTACATGACCACTTGA 226 GGCCACACGCTGCCCTAAAGTGT 426 TAGGGAAGAGAAGGACATATGATGGCCACACGCTGCCCT TCGTGTA AAAGTGTTCGTGTATTGACTAGTACATGACCACTTGA 227 GTTCTGACTGGGTGTGGTGCTGC 427 TAGGGAAGAGAAGGACATATGATGTTCTGACTGGGTGTG ACTGTCA GTGCTGCACTGTCATTGACTAGTACATGACCACTTGA 228 GGCAACGCACATCGTATCACGCA 428 TAGGGAAGAGAAGGACATATGATGGCAACGCACATCGTA TCGGACC TCACGCATCGGACCTTGACTAGTACATGACCACTTGA 229 GTCATGCGCGGACATTCAAGTTG 429 TAGGGAAGAGAAGGACATATGATGTCATGCGCGGACATT GCGTGGA CAAGTTGGCGTGGATTGACTAGTACATGACCACTTGA 230 CCGTAGCGACATCAAGCGGTGGT 430 TAGGGAAGAGAAGGACATATGATCCGTAGCGACATCAAG GTGCGTG CGGTGGTGTGCGTGTTGACTAGTACATGACCACTTGA 231 GTACGACGCGGACCTTCAAGTAG 431 TAGGGAAGAGAAGGACATATGATGTACGACGCGGACCTT GCGTGTA CAAGTAGGCGTGTATTGACTAGTACATGACCACTTGA 232 GACCTGACTGTGCCTATCGAGTG 432 TAGGGAAGAGAAGGACATATGATGACCTGACTGTGCCTA CGTGATG TCGAGTGCGTGATGTTGACTAGTACATGACCACTTGA 233 TGGCCGATCGACCCTATCAAGTG 433 TAGGGAAGAGAAGGACATATGATTGGCCGATCGACCCTA CAGCATG TCAAGTGCAGCATGTTGACTAGTACATGACCACTTGA 234 GTTCCGAGCTGGATGTGGCCTGT 434 TAGGGAAGAGAAGGACATATGATGTTCCGAGCTGGATGT GCTATGC GGCCTGTGCTATGCTTGACTAGTACATGACCACTTGA 235 GGCATGCGATGGATGTGTGCGTG 435 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGT TATTAGC GTGCGTGTATTAGCTTGACTAGTACATGACCACTTGA 236 GTACGCATCGTCCCGTCATGTGG 436 TAGGGAAGAGAAGGACATATGATGTACGCATCGTCCCGT TTCCGTA CATGTGGTTCCGTATTGACTAGTACATGACCACTTGA 237 GGCATTGCGCGCCTAGCAAGTTG 437 TAGGGAAGAGAAGGACATATGATGGCATTGCGCGCCTAG ACGTGTA CAAGTTGACGTGTATTGACTAGTACATGACCACTTGA 238 GGACGCACGCAGACCTTCAAGTC 438 TAGGGAAGAGAAGGACATATGATGGACGCACGCAGACCT GGCCATG TCAAGTCGGCCATGTTGACTAGTACATGACCACTTGA 239 GTGCTGCATGAGCGGTGTGCGTG 439 TAGGGAAGAGAAGGACATATGATGTGCTGCATGAGCGGT TACGACG GTGCGTGTACGACGTTGACTAGTACATGACCACTTGA 240 GTCATGCTCGACACTATCAGGTG 440 TAGGGAAGAGAAGGACATATGATGTCATGCTCGCACTAT TGCATGGA CAGGTGTGCATGGATTGACTAGTACATGACCACTTGA 241 GTGCGCGGCTTGCCTTCACGTGA 441 TAGGGAAGAGAAGGACATATGATGTGCGCGGCTTGCCTT TCGTGTA CACGTGATCGTGTATTGACTAGTACATGACCACTTGA 242 GTCATACGATGGGTGTGGTATGT 442 TAGGGAAGAGAAGGACATATGATGTCATACGATGGGTGT GTACGTA GGTATGTGTACGTATTGACTAGTACATGACCACTTGA 243 GCATGCGTTGGACTTGTCTGGCT 443 TAGGGAAGAGAAGGACATATGATGCATGCGTTGGACTTG GTGGGTG TCTGGCTGTGGGTGTTGACTAGTACATGACCACTTGA 244 TGCGTCGTATGTGCGGCTCGGAT 444 TAGGGAAGAGAAGGACATATGATTGCGTCGTATGTGCGG GTGTGTC CTCGGATGTGTGTCTTGACTAGTACATGACCACTTGA 245 GGACGCAGCTTGCCTACTGGTGG 445 TAGGGAAGAGAAGGACATATGATGGACGCAGCTTGCCTA TCACGTA CTGGTGGTCACGTATTGACTAGTACATGACCACTTGA 246 GGCCATCGATGGGTGTGGCTGTA 446 TAGGGAAGAGAAGGACATATGATGGCCATCGATGGGTGT CTTGACA GGCTGTACTTGACATTGACTAGTACATGACCACTTGA 247 GCGTGTCAGCAATACGTCCTCAT 447 TAGGGAAGAGAAGGACATATGATGCGTGTCAGCAATACG CTGCCCG TCCTCATCTGCCCGTTGACTAGTACATGACCACTTGA 248 GTGCGATCGTACCTATCAATGGT 448 TAGGGAAGAGAAGGACATATGATGTGCGATCGTACCTAT CATCGTA CAATGGTCATCGTATTGACTAGTACATGACCACTTGA 249 GGCATGCGATGGATGGGGGCTGG 449 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGG GGCAGTC GGGCTGGGGCAGTCTTGACTAGTACATGACCACTTGA 250 GGCCGACGATGGCGTAGCGTCTG 450 TAGGGAAGAGAAGGACATATGATGGCCGACGATGGCGTA TACTGTT GCGTCTGTACTGTTTTGACTAGTACATGACCACTTGA 251 TGGCCGATCATCCCTCAAGTTGG 451 TAGGGAAGAGAAGGACATATGATTGGCCGATCATCCCTC CGTGTGC AAGTTGGCGTGTGCTTGACTAGTACATGACCACTTGA 252 GGCCGTACGATGGATGTGGGATG 452 TAGGGAAGAGAAGGACATATGATGGCCGTACGATGGATG GTCTAGC TGGGATGGTCTAGCTTGACTAGTACATGACCACTTGA 253 GGCACAAACGGACCGACAAGTGC 453 TAGGGAAGAGAAGGACATATGATGGCACAAACGGACCGA GCATGGA CAAGTGCGCATGGATTGACTAGTACATGACCACTTGA 254 GTACGGAACGGAACAACAAGGGC 454 TAGGGAAGAGAAGGACATATGATGTACGGAACGGAACAA AGGCATG CAAGGGCAGGCATGTTGACTAGTACATGACCACTTGA 255 GGACGCACATCCCGTTCATGTGT 455 TAGGGAAGAGAAGGACATATGATGGACGCACATCCCGTT GCATGTA CATGTGTGCATGTATTGACTAGTACATGACCACTTGA 256 GGCCAAGCTGGATGTGTTCAGGT 456 TAGGGAAGAGAAGGACATATGATGGCCAAGCTGGATGTG CACGACG TTCAGGTCACGACGTTGACTAGTACATGACCACTTGA 257 GGCCTGCGATGGATGTGTGCGTG 457 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TA GTGCGTGTATTGACTAGTACATGACCACTTGA 258 CGTGCGCGAGACATGTCCATCGG 458 TAGGGAAGAGAAGGACATATGATCGTGCGCGAGACATGG TTCGTG TCCATCGGTTCGTGTTGACTAGTACATGACCACTTGA 259 GTCATGCGCTGGGTGTGGCCTGT 459 TAGGGAAGAGAAGGACATATGATGTCATGCGCTGGGTGT TGTAGGC GGCCTGTTGTAGGCTTGACTAGTACATGACCACTTGA 260 GTCGCGATGAGCTAGCATGTGCG 460 TAGGGAAGAGAAGGACATATGATGTCGCGATGAGCTAGC TTGTGTA ATGTGCGTTGTGTATTGACTAGTACATGACCACTTGA 261 GTGCTACGATGGCTGTGGGCGTG 461 TAGGGAAGAGAAGGACATATGATGTGCTACGATGGCTGT ATGCGTA GGGCGTGATGCGTATTGACTAGTACATGACCACTTGA 262 GACGCTGCGTTCCCTATCATGTG 462 TAGGGAAGAGAAGGACATATGATGACGCTGCGTTCCCTA CGGCATG TCATGTGCGGCATGTTGACTAGTACATGACCACTTGA 263 GTTCGCGCGACACCTATCAATGT 463 TAGGAAGAGAAGGACATATGATGTCCGCGCGACACCTAT GGACGTG CAATGTGGACGTGTTGACTAGTACATGACCACTTGA 264 GCACGACTCGCACCCTATCATGA 464 TAGGGAAGAGAAGGACATATGATGCACGACTCGCACCCT GGCCATG ATCATGAGGCCATGTTGACTAGTACATGACCACTTGA 265 GTCATGAAACGAGCCTACACGTG 465 TAGGGAAGAGAAGGACATATGATGTCATGAAACGAGCCT GTGCATG ACACGTGGTGCATGTTGACTAGTACATGACCACTTGA 266 GGACGCGATGGGCGTGGGTATGC 466 TAGGGAAGAGAAGGACATATGATGGACGCGATGGGCGTG ACTTGGC GGTATGCACTTGGCTTGACTAGTACATGACCACTTGA 267 GTACTGCGATGGCTTAGCAAAGT 467 TAGGGAAGAGAAGGACATATGATGTACTGCGATGGCTTA GCGACATG GCAAAGTGCGACATGTTGACTAGTACATGACCACTTGA 268 TGCCCTGGCAATGCGATGTTCGA 468 TAGGGAAGAGAAGGACATATGATTGCCCTGGCAATGCGA TGCGACC TGTTCGATGCGACCTTGACTAGTACATGACCACTTGA 269 GTACGCGACGTCCCTGAGAGTGT 469 TAGGGAAGAGAAGGACATATGATGTACGCGACGTCCCTG GCAGGTA AGAGTGTGCAGGTATTGACTAGTACATGACCACTTGA 270 GTGCGCCGATATCCCTTCACAGT 470 TAGGGAAGAGAAGGACATATGATGTGCGCCGATATCCCT TGGCATG TCACAGTTGGCATGTTGACTAGTACATGACCACTTGA 271 GGCCGACGATGGATGGGAGGCAT 471 TAGGGAAGAGAAGGACATATGATGGCCGACGATGGATGG GACTGGC GAGGCATGACTGGCTTGACTAGTACATGACCACTTGA 272 GTACGCGCTGGTCCCGTATCATG 472 TAGGGAAGAGAAGGACATATGATGTACGCGCTGGTCCCG TGCGTCA TATCATGTGCGTCATTGACTAGTACATGACCACTTGA 273 GGCCTCGATGGATGTGGTGGTGC 473 TAGGGAAGAGAAGGACATATGATGGCCTCGATGGATGTG TGTCA GTGGTGCTGTCATTGACTAGTACATGACCACTTGA 274 GGCCGAACTGGATGGGGGCATTA 474 TAGGGAAGAGAAGGACATATGATGGCCGAACTGGATGGG CTGCGGC GGCATTACTGCGGCTTGACTAGTACATGACCACTTGA 275 GTCACGGAACGAAGCCTATCAAG 475 TAGGGAAGAGAAGGACATATGATGTCACGGAACGAAGCC TGCGACA TATCAAGTGCGACATTGACTAGTACATGACCACTTGA 276 GGCACGGAGGATGGACGTTCTGC 476 TAGGGAAGAGAAGGACATATGATGGCACGGAGGATGGAC CTTGGTC GTTCTGCCTTGGTCTTGACTAGTACATGACCACTTGA 277 GCAACTGCACGCATTGGACCGCA 477 TAGGGAAGAGAAGGACATATGATGCAACTGCACGCATTG CGTCACA GACCGCACGTCACATTGACTAGTACATGACCACTTGA 278 GTGCTGAGCTGGGAGTGGTGGTG 478 TAGGGAAGAGAAGGACATATGATGTGCTGAGCTGGGAGT CTTTGGC GGTGGTGCTTTGGCTTGACTAGTACATGACCACTTGA 279 GTCTGCCGATGGATTGGTGTACG 479 TAGGGAAGAGAAGGACATATGATGTCTGCCGATGGATGT CAGACG GGTGTACGCAGACGTTGACTAGTACATGACCACTTGA 280 GTACACGATGCACCTTCAAGTTG 480 TAGGGAAGAGAAGGACATATGATGTACACGATGCACCTT TGATGTA CAAGTTGTGATGTATTGACTAGTACATGACCACTTGA 281 GGACGCGTCGACCTTCAAGTGTG 481 TAGGGAAGAGAAGGACATATGATGGACGCGTCGACCTTC CCGTGGA AAGTGTGCCGTGGATTGACTAGTACATGACCACTTGA 282 GTCATTCGCTGGATGTGTTGATG 482 TAGGGAAGAGAAGGACATATGATGTCATTCGCTGGATGT TCTGGTC GTTGATGTCTGGTCTTGACTAGTACATGACCACTTGA 283 CGCATGGGACGTACTGACCGGAT 483 TAGGGAAGAGAAGGACATATGATCGCATGGGACGTACTG CGTGTCA ACCGGATCGTGTCATTGACTAGTACATGACCACTTGA 284 GGCCACGATGGATGAGGACATGA 484 TAGGGAAGAGAAGGACATATGATGGCCACGATGGATGAG CTGGTTG GACATGACTGGTTGTTGACTAGTACATGACCACTTGA 285 GTGCGACACGTGTTCCCGTTCAA 485 TAGGGAAGAGAAGGACATATGATGTGCGACACGTGTTCC GTTGGGC CGTTCAAGTTGGGCTTGACTAGTACATGACCACTTGA 286 CACGACAGCGTTAGCAGGCCATG 486 TAGGGAAGAGAAGGACATATGATCACGACAGCGTTAGCA CGACACG GGCCATGCGACACGTTGACTAGTACATGACCACTTGA 287 GTCGTGCGTGCCCTATCAAGTCG 487 TAGGGAAGAGAAGGACATATGATGTCGTGCGTGCCCTAT GTCTGTA CAAGTCGGTCTGTATTGACTAGTACATGACCACTTGA 288 GGCATGCGATGGGTGTGTTCTGG 488 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGGTGT CGACGGC GTTCTGGCGACGGCTTGACTAGTACATGACCACTTGA 289 GTCTGAGCGCAACCTCGTGGACT 489 TAGGGAAGAGAAGGACATATGATGTCTGAGCGCAACCTC GTGCGTG GTGGACTGTGCGTGTTGACTAGTACATGACCACTTGA 290 GGCCGCGTCTGGATGTGGTTTTG 490 TAGGGAAGAGAAGGACATATGATGGCCGCGTCTGGATGT TCGCGTC GGTTTTGTCGCGTCTTGACTAGTACATGACCACTTGA 291 CCGTGTTGCGTGTCCAGTCTCGT 491 TAGGGAAGAGAAGGACATATGATCCGTGTTGCGTGTCCA TGCGCG GTCTCGTTGCGCGTTGACTAGTACATGACCACTTGA 292 GGCCGGCGATGGATGTGGTTGTG 492 TAGGGAAGAGAAGGACATATGATGGCCGGCGATGGATGT CTTGTTT GGTTGTGCTTGTTTTTGACTAGTACATGACCACTTGA 293 GTGCGATACATCCCAACCTCCCG 493 TAGGGAAGAGAAGGACATATGATGTGCGATACATCCCAAC TGTGGC CCTCCCGTGTGGCTTGACTAGTACATGACCACTTGA 294 GCCGCAACGACTGAGGGGTGTAT 494 TAGGGAAGAGAAGGACATATGATGCCGCAACGACTGAGG GTACGCG GGTGTATGTACGCGTTGACTAGTACATGACCACTTGA 295 GGACGCGGATGAGCTTCGAGTGA 495 TAGGGAAGAGAAGGACATATGATGGACGCGGATGAGCTT CGTGTAC CGAGTGACGTGTACTTGACTAGTACATGACCACTTGA 296 GTCGTGACTGGCGTAGCTGGTAG 496 TAGGGAAGAGAAGGACATATGATGTCGTGACTGGCGTAG TGCTAGG CTGGTAGTGCTAGGTTGACTAGTACATGACCACTTGA

TABLE 4 Aptamers against tree nut antigen SEQ ID NO. Unique Sequence (5′-3′) SEQ ID NO. Full sequence including primers (5′-3′) 497 GTCATTCCGCATCCTACACGTGG 597 TAGGGAAGAGAAGGACATATGATGTCATTCCGCATCCTA GCACGTA CACGTGGGCACGTATTGACTAGTACATGACCACTTGA 498 GGCATGCACGCACCTACAGTGGG 598 TAGGGAAGAGAAGGACATATGATGGCATGCACGCACCTA TATGGA CACGTGGGTATGGATTGACTAGTACATGACCACTTGA 499 GGCCTGCGATGGATGTGTGCGTG 599 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATTAGC GTGCGTGTATTAGCTTGACTAGTACATGACCACTTGA 500 GCACGACTCGCACCCTATCATGA 600 TAGGGAAGAGAAGGACATATGATGCACGACTCGCACCCT GGCCATG ATCATGAGGCCATGTTGACTAGTACATGACCACTTGA 501 GTCATGCCATCCCTTCGAGTGTG 601 TAGGGAAGAGAAGGACATATGATGTCATGCCATCCCTTC ACAGGTA GAGTGTGACAGGTATTGACTAGTACATGACCACTTGA 502 GGCCTGCGATGGATGAGGTGCTG 602 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGA CACTAGT GGTGCTGCACTAGTTTGACTAGTACATGACCACTTGA 503 GGACGCAGCTTGCCTACTGGTGG 603 TAGGGAAGAGAAGGACATATGATGGACGCAGCTTGCCTA TCACGTA CTGGTGGTCACGTATTGACTAGTACATGACCACTTGA 504 GGCCAATGCGCCCCTTCATGTTG 604 TAGGGAAGAGAAGGACATATGATGGCCAATGCGCCCCTT TCGTGTA CATGTTGTCGTGTATTGACTAGTACATGACCACTTGA 505 GTGCGCACGATGGATGTGGATGG 605 TAGGGAAGAGAAGGACATATGATGTGCGCACGATGGATG CCAGTCT TGGATGGCCAGTCTTTGACTAGTACATGACCACTTGA 506 GTCATGCGCGGACATTCAAGTTG 606 TAGGGAAGAGAAGGACATATGATGTCATGCGCGGACATT GCGTGGA CAAGTTGGCGTGGATTGACTAGTACATGACCACTTGA 507 CCGCACGTAGCCCTATCAGTGGT 607 TAGGGAAGAGAAGGACATATGATCCGCACGTAGCCCTAT GCATGCA CAGTGGTGCATGCATTGACTAGTACATGACCACTTGA 508 GGCATGCGCTGGGTAGTGATCAC 608 TAGGGAAGAGAAGGACATATGATGGCATGCGCTGGGTAG GTACGGGT TGATCACGTACGGTTTGACTAGTACATGACCACTTGA 509 GGCCTGCGATGGATGTGGGCTAG 609 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGATGT TATGGGC GGGCTAGTATGGGCTTGACTAGTACATGACCACTTGA 510 GTGCGACCGACCCTATCAGGTGC 610 TAGGGAAGAGAAGGACATATGATGTGCGACCGACCCTAT TCATGTA CAGGTGCTCATGTATTGACTAGTACATGACCACTTGA 511 GTACTGCACTGCCCTACACGTGG 611 TAGGGAAGAGAAGGACATATGATGTACTGCACTGCCCTA GAATGGA CACGTGGGAATGGATTGACTAGTACATGACCACTTGA 512 GGCCGACCTGGATGTGAGCATGC 612 TAGGGAAGAGAAGGACATATGATGGCCGACCTGGATGTG ATCTAGT AGCATGCATCTAGTTTGACTAGTACATGACCACTTGA 513 CGCACCGTCGATACGTCATGCAC 613 TAGGGAAGAGAAGGACATATGATCGCACCGTCGATACGT GCTGACA CATGCACGCTGACATTGACTAGTACATGACCACTTGA 514 GGCATGCGATGGATGGGGGCTGG 614 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGG GGCAGTC GGGCTGGGGCAGTCTTGACTAGTACATGACCACTTGA 515 GACGGTGCGTCCTAAAGTGCTCA 615 TAGGGAAGAGAAGGACATATGATGACGGTGCGTCCTAAA GTGCGTG GTGCTCAGTGCGTGTTGACTAGTACATGACCACTTGA 516 GTACGCATCGTCCCGTCATGTGG 616 TAGGGAAGAGAAGGACATATGATGTACGCATCGTCCCGT TTCCGTA CATGTGGTTCCGTATTGACTAGTACATGACCACTTGA 517 GTGCGACCTGACCTAGCAAGCGG 617 TAGGGAAGAGAAGGACATATGATGTGCGACCTGACCTAG TAGTGTA CAAGCGGTAGTGTATTGACTAGTACATGACCACTTGA 518 GTACGACGCGGACCTTCAAGTAG 618 TAGGGAAGAGAAGGACATATGATGTACGACGCGGACCTT GCGTGTA CAAGTAGGCGTGTATTGACTAGTACATGACCACTTGA 519 GGCCAAGCTGACCGTAAAGGCAG 619 TAGGGAAGAGAAGGACATATGATGGCCAAGCTGACCGTA GCAGTGTA AAGGCAGGCGTGTATTGACTAGTACATGACCACTTGA 520 GTACGCGACGTCCCTGAGAGTGT 620 TAGGGAAGAGAAGGACATATGATGTACGCGACGTCCCTG GCAGGTA AGAGTGTGCAGGTATTGACTAGTACATGACCACTTGA 521 GTCAGTCGATGGATGTGGGTTGT 621 TAGGGAAGAGAAGGACATATGATGTCAGTCGATGGATGT GCTCGTC GGGTTGTGCTCGTCTTGACTAGTACATGACCACTTGA 522 CGCACCGTCAAGCGGGAAGGCAC 622 TAGGGAAGAGAAGGACATATGATCGCACCGTCAAGCGGG TTTGGTG AAGGCACTTTGGTGTTGACTAGTACATGACCACTTGA 523 GGACGCACGCAGACCTTCAAGTC 623 TAGGGAAGAGAAGGACATATGATGGACGCACGCAGACCT GGCCATG TCAAGTCGGCCATGTTGACTAGTACATGACCACTTGA 524 CCGTAGCGACATCAAGCGGTGGT 624 TAGGGAAGAGAAGGACATATGATCCGTAGCGACATCAAG GTGCGTG CGGTGGTGTGCGTGTTGACTAGTACATGACCACTTGA 525 GTGCGCGGCTTGCCTTCACGTGA 625 TAGGGAAGAGAAGGACATATGATGTGCGCGGCTTGCCTT TCGTGTA CACGTGATCGTGTATTGACTAGTACATGACCACTTGA 526 GGCCTGATCGAACCTAGAGAGTG 626 TAGGGAAGAGAAGGACATATGATGGCCTGATCGAACCTA GCGTGGA GAGAGTGGCGTGGATTGACTAGTACATGACCACTTGA 527 GGACGCATCGCCCCTTCGAGTGG 627 TAGGGAAGAGAAGGACATATGATGGACGCATCGCCCCTT ACAGGTA CGAGTGGACAGGTATTGACTAGTACATGACCACTTGA 528 GTACGCACGATGAGCGCCAAGTG 628 TAGGGAAGAGAAGGACATATGATGTACGCACGATGAGCG ACATGGA CCAAGTGACATGGATTGACTAGTACATGACCACTTGA 529 GGCATGCGATGGATGTGGTGTAC 629 TAGGGAAGAGAAGGACATATGATGGCATGCGATGGATGT CCAGTCC GGTGTACCCAGTCCTTGACTAGTACATGACCACTTGA 530 GGACGGAACGTGAGGGCAAGTAC 630 TAGGGAAGAGAAGGACATATGATGGACGGAACGTGAGGG GTGCTCG CAAGTACGTGCTCGTTGACTAGTACATGACCACTTGA 531 CCATCGCGTCACATCATGTGTGT 631 TAGGGAAGAGAAGGACATATGATCCATCGCGTCACTATC CACTGC ATGTGTGTCACGTATTGACTAGTACATGACCACTTGA 532 GTCGTGACTGGCTAGCTGGACAT 632 TAGGGAAGAGAAGGACATATGATGTCGTGACTGGCTAGC GCACTGC TGGACATGCACTGCTTGACTAGTACATGACCACTTGA 533 GGACTGCGCGTGACCTATCAATG 633 TAGGGAAGAGAAGGACATATGATGGACTGCGCGTGACCT GCATGTA ATCAATGGCATGTATTGACTAGTACATGACCACTTGA 534 GACCTGACTGTGCCTATCGAGTG 634 TAGGGAAGAGAAGGACATATGATGACCTGACTGTGCCTA CGTGATG TCGAGTGCGTGATGTTGACTAGTACATGACCACTTGA 535 AATGCGGCATGAACGGACCTACA 635 TAGGGAAGAGAAGGACATATGATAATGCGGCATGAACGG CGTGGGC ACCTACACGTGGGCTTGACTAGTACATGACCACTTGA 536 GCATTGGACGATCGTGCCCTACA 636 TAGGGAAGAGAAGGACATATGATGCATTGGACGATCGTG CGTGGGC CCCTACACGTGGGCTTGACTAGTACATGACCACTTGA 537 GGCCACACGCTGCCCTAAAGTGT 637 TAGGGAAGAGAAGGACATATGATGGCCACACGCTGCCCT TCGTGTA AAAGTGTTCGTGTATTGACTAGTACATGACCACTTGA 538 GTACGGAACGGAACAACAAGGGC 638 TAGGGAAGAGAAGGACATATGATGTACGGAACGGAACAA AGGCATG CAAGGGCAGGCATGTTGACTAGTACATGACCACTTGA 539 GGCCAGATCGACATAGCGAGTGA 639 TAGGGAAGAGAAGGACATATGATGGCCAGATCGACATAG GAGTGTA CGAGTGAGAGTGTATTGACTAGTACATGACCACTTGA 540 GTCATGCGCGTACCATCGAGGGG 640 TAGGGAAGAGAAGGACATATGATGTCATGCGCGTACCAT GCGTGGA CGAGGGGGCGTGGATTGACTAGTACATGACCACTTGA 541 GCACGCCGATGCCCTCATGTGGC 641 TAGGGAAGAGAAGGACATATGATGCACGCCGATGCCCTC CGTGGA ATGTGGCCGTGGATTGACTAGTACATGACCACTTGA 542 GCACTGAGCGTACGTATCAGCGG 642 TAGGGAAGAGAAGGACATATGATGCACTGAGCGTACGTA GCACGTA TCAGCGGGCACGTATTGACTAGTACATGACCACTTGA 543 GTGCTGAGCTGGGAGTGGTGGTG 643 TAGGGAAGAGAAGGACATATGATGTGCTGAGCTGGGAGT CTTTGGC GGTGGTGCTTTGGCTTGACTAGTACATGACCACTTGA 544 GTGCTGCGATGGATTGGGAGTGT 644 TAGGGAAGAGAAGGACATATGATGTGCTGCGATGGATTG CTTTGGC GGAGTGTCTTTGGCTTGACTAGTACATGACCACTTGA 545 GTACGCGGCTGGATACAAGTACG 645 TAGGGAAGAGAAGGACATATGATGTACGCGGCTGGATAC GCATGGA AAGTACGGCATGGATTGACTAGTACATGACCACTTGA 546 GGACGCGATGGATGTGGACGGTG 646 TAGGGAAGAGAAGGACATATGATGGACGCGATGGATGTG TGGTAGT GACGGTGTGGTAGTTTGACTAGTACATGACCACTTGA 547 GTCATGCACGAACACTATCATGG 647 TAGGGAAGAGAAGGACATATGATGTCATGCACGAACACT CGGCATG ATCATGGCGGCATGTTGACTAGTACATGACCACTTGA 548 GTCATGCTCGCACTATCAGGTGT 648 TAGGGAAGAGAAGGACATATGATGTCATGCTCGCACTAT GCATGGA CAGGTGTGCATGGATTGACTAGTACATGACCACTTGA 549 GGCCTGACTGGGTGTGGTTAGGA 649 TAGGGAAGAGAAGGACATATGATGGCCTGACTGGGTGTG ACGCGTC GTTAGGAACGCGTCTTGACTAGTACATGACCACTTGA 550 GTGCTCGCAAGACCTACACGTGG 650 TAGGGAAGAGAAGGACATATGATGTGCTCGCAAGACCTA ACGTGGA CACGTGGACGTGGATTGACTAGTACATGACCACTTGA 551 GGCACAAACGGACCGACAAGTGC 651 TAGGGAAGAGAAGGACATATGATGGCACAAACGGACCGA GCATGGA CAAGTGCGCATGGATTGACTAGTACATGACCACTTGA 552 TCGATCGATCCGTCAAGCAGGCA 652 TAGGGAAGAGAAGGACATATGATTCGATCGATCCGTCAA CGTGTCA GCAGGCACGTGTCATTGACTAGTACATGACCACTTGA 553 GGCATTGCGCGCCTAGCAAGTTG 653 TAGGGAAGAGAAGGACATATGATGGCATTGCGCGCCTAG ACGTGTA CAAGTTGACGTGTATTGACTAGTACATGACCACTTGA 554 GGACGCGTCGACTTCAAGTGTGC 654 TAGGGAAGAGAAGGACATATGATGGACGCGTCGACCTTC CGTGGA AAGTGTGCCGTGGATTGACTAGTACATGACCACTTGA 555 CCGCATCGGACCGATCAAGGCAG 655 TAGGGAAGAGAAGGACATATGATCCGCATCGGACCGATC GCTTGGA AAGGCAGGCTTGGATTGACTAGTACATGACCACTTGA 556 TGGCCAAGCGACCTAGCAAGTGT 656 TAGGGAAGAGAAGGACATATGATTGGCCAAGCGACCTAG GCTCATG CAAGTGTGCTCATGTTGACTAGTACATGACCACTTGA 557 GGCATGCGATGAACGAGGCATGA 657 TAGGGAAGAGAAGGACATATGATGGCATGCGATGAACGA TGCGTCA GGCATGATGCGTCATTGACTAGTACATGACCACTTGA 558 GTACGACGCGAGCTAGCAAGGAG 658 TAGGGAAGAGAAGGACATATGATGTACGACGCGAGCTAG GCGTGTA CAAGGAGGCGTGTATTGACTAGTACATGACCACTTGA 559 GGCATGCACGCACCTACACGTGG 659 TAGGGAAGAGAAGGACATATGATGGCATGCACGCACCTA GCACGTA CACGTGGGCACGTATTGACTAGTACATGACCACTTGA 560 CCATATGGCAGTGCGATGGCTTC 660 TAGGGAAGAGAAGGACATATGATCCATATGGCAGTGCGA GCTGGTC TGGCTTCGCTGGTCTTGACTAGTACATGACCACTTGA 561 GTCATGCGCTGGGTGTGGCCTGT 661 TAGGGAAGAGAAGGACATATGATGTCATGCGCTGGGTGT TGTAGGC GGCCTGTTGTAGGCTTGACTAGTACATGACCACTTGA 562 GTGCTGCCTGACCCACGTGGACT 662 TAGGGAAGAGAAGGACATATGATGTGCTGCCTGACCCAC TGCACTA GTGGACTTGCACTATTGACTAGTACATGACCACTTGA 563 GGACTGACGAGCCGTTCATGTGG 663 TAGGGAAGAGAAGGACATATGATGGACTGACGAGCCGTT TTGTGGA CATGTGGTTGTGGATTGACTAGTACATGACCACTTGA 564 CGCAACGGTGACGAGCAGTGAGT 664 TAGGGAAGAGAAGGACATATGATCGCAACGGTGACGAGC GCATGTA AGTGAGTGCATGTATTGACTAGTACATGACCACTTGA 565 GGACGGATCGAACCTACAAGTTG 665 TAGGGAAGAGAAGGACATATGATGGACGGATCGAACCTA TCGTGGA CAAGTTGTCGTGGATTGACTAGTACATGACCACTTGA 566 GTCGTGAGCTGGAAGGAGAGTGG 666 TAGGGAAGAGAAGGACATATGATGTCGTGAGCTGGAAGG GTACGTA AGAGTGGGTACGTATTGACTAGTACATGACCACTTGA 567 GTCATTGTCGGATGTGAGCATGT 667 TAGGGAAGAGAAGGACATATGATGTCATTGTCGGATGTG TTCTCGGC AGCATGTTCTCGGCTTGACTAGTACATGACCACTTGA 568 GCGTGTCAGCAATACGTCCTCAT 668 TAGGGAAGAGAAGGACATATGATGCGTGTCAGCAATACG CTGCCCG TCCTCATCTGCCCGTTGACTAGTACATGACCACTTGA 569 GTCACGGAACGAAGCCTATCAAG 669 TAGGGAAGAGAAGGACATATGATGTCACGGAACGAAGCC TGCGACA TATCAAGTGCGACATTGACTAGTACATGACCACTTGA 570 GCGACAGCGACATACGATCTGCT 670 TAGGGAAGAGAAGGACATATGATGCGACAGCGACATACG CTGCGTC ATCTGCTCTGCGTCTTGACTAGTACATGACCACTTGA 571 GTTCGCGCGACACCTATCAATGT 671 TAGGGAAGAGAAGGACATATGATGTTCGCGCGACACCTA GGACGTG TCAATGTGGACGTGTTGACTAGTACATGACCACTTGA 572 GACACGCCGATGAGCCTAGCCTG 672 TAGGGAAGAGAAGGACATATGATGACACGCCGATGAGCC TACGACG TAGCCTGTACGACGTTGACTAGTACATGACCACTTGA 573 GGCCGAACTGGATGGGGGCATTA 673 TAGGGAAGAGAAGGACATATGATGGCCGAACTGGATGGG CTGCGGC GGCATTACTGCGGCTTGACTAGTACATGACCACTTGA 574 GTACGCCTCGGAGCTAGCAGGTG 674 TAGGGAAGAGAAGGACATATGATGTACGCCTCGGAGCTA GTGTGGA GCAGGTGGTGTGGATTGACTAGTACATGACCACTTGA 575 GGCCAAGCTGGATGTGTTCAGGT 675 TAGGGAAGAGAAGGACATATGATGGCCAAGCTGGATGTG CACGACG TTCAGGTCACGACGTTGACTAGTACATGACCACTTGA 576 GTCATGCTCTGGGTGTGCGAATG 676 TAGGGAAGAGAAGGACATATGATGTCATGCTCTGGGTGT TGGTAGG GCGAATGTGGTAGGTTGACTAGTACATGACCACTTGA 577 GTCACTGTGCCTGACCGTCAAGT 677 TAGGGAAGAGAAGGACATATGATGTCACTGTGCCTGACC TGCGGCA GTCAAGTTGCGGCATTGACTAGTACATGACCACTTGA 578 CGACGCAATCGGACACTGGACAT 678 TAGGGAAGAGAAGGACATATGATCGACGCAATCGGACAC GCGCAGA TGGACATGCGCAGATTGACTAGTACATGACCACTTGA 579 GCACGTACGCCTTGCCTATCTGT 679 TAGGGAAGAGAAGGACATATGATGCACGTACGCCTTGCC GCTCATG TATCTGTGCTCATGTTGACTAGTACATGACCACTTGA 580 GTGCGCCGATATCCCTTCACAGT 680 TAGGGAAGAGAAGGACATATGATGTGCGCCGATATCCCT TGGCATG TCACAGTTGGCATGTTGACTAGTACATGACCACTTGA 581 CATGTGTCGACTCGCCCTATCAT 681 TAGGGAAGAGAAGGACATATGATCATGTGTCGACTCGCC GCGGTCA CTATCATGCGGTCATTGACTAGTACATGACCACTTGA 582 GGACGCACATCCCGTTCATGTGT 682 TAGGGAAGAGAAGGACATATGATGGACGCACATCCCGTT GCATGTA CATGTGTGCATGTATTGACTAGTACATGACCACTTGA 583 GGACTCGCGTCACTATCACGGGG 683 TAGGGAAGAGAAGGACATATGATGGACTCGCGTCACTAT GCAGGTA CACGGGGGCAGGTATTGACTAGTACATGACCACTTGA 584 GCTTCGATGGATGCTGGGCAGGC 684 TAGGGAAGAGAAGGACATATGATGCTTCGATGGATGCTG ACGCAGT GGCAGGCACGCAGTTTGACTAGTACATGACCACTTGA 585 GACATTCGCTGGATGTGGGGATG 685 TAGGGAAGAGAAGGACATATGATGACATTCGCTGGATGT CACTGTC GGGGATGCACTGTCTTGACTAGTACATGACCACTTGA 586 TGGCCGATCGACCCTATCAAGTG 686 TAGGGAAGAGAAGGACATATGATTGGCCGATCGACCCTA CAGCATG TCAAGTGCAGCATGTTGACTAGTACATGACCACTTGA 587 GTGCGACCGACCCTATCAAGTAC 687 TAGGGAAGAGAAGGACATATGATGTGCGACCGACCCTAT GTCA CAAGTACGTCATTGACTAGTACATGACCACTTGA 588 GTGCTGAACGTACCGATTCAAGT 688 TAGGGAAGAGAAGGACATATGATGTGCTGAACGTACCGA GTGCGTG TTCAAGTGTGCGTGTTGACTAGTACATGACCACTTGA 589 GGCCTGCGATGGAATGTGCGAAT 689 TAGGGAAGAGAAGGACATATGATGGCCTGCGATGGAATG GTACGCA TGCGAATGTACGCATTGACTAGTACATGACCACTTGA 590 CTCATGCGGACCGAACTGGATGT 690 TAGGGAAGAGAAGGACATATGATCTCATGCGGACCGAAC GTGCATG TGGATGTGTGCATGTTGACTAGTACATGACCACTTGA 591 GTTCTGACTGGTGTGGTGCTGCA 691 TAGGGAAGAGAAGGACATATGATGTTCTGACTGGGTGTG CTGTCA GTGCTGCACTGTCATTGACTAGTACATGACCACTTGA 592 GTCGTGCGTGCCCTATCAAGTCG 692 TAGGGAAGAGAAGGACATATGATGTCGTGCGTGCCCTAT GTCTGTA CAAGTCGGTCTGTATTGACTAGTACATGACCACTTGA 593 GGCCGAATGACCGTCTCATGTGA 693 GCATGGA 594 GGTCCGAACGCACCTCATGTGTG 694 TCGTGTA 595 GGTCTGCGCGTACCGTCAAGTGC 695 GAATGGA 596 GTCGTGAGCGGGTGTGGGACTGG 696 ACGCAGT

4. SPN-Complement Complexes

In some embodiments, SPN-complement complexes are provided. A nucleic acid sequence that is complementary to a portion of the sequence of a signaling polynucleotide (SPN) (e.g., either the 5′end or 3′end sequence of the SPN) is hybridized with the corresponding SPN sequence, forming a SPN-complement complex. In some aspects, the complementary sequence may contain about 5 to 20 nucleotide residues, or about 5 to 10 nucleotide residues, or about 10 to 15 nucleotide residues, or about 10-20 nucleotide residues. In particular, it may contain 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, or 20 nucleotide residues. In one embodiment, the complementary sequence contains 5 nucleotide residues. In another embodiment, the complementary sequence contains 10 nucleotide residues. In some aspects, the complementary sequence may be at least 100% complementary to the SPN sequence, or at least 99% complementary to the SPN sequence, or at least 95% complementary to the SPN sequence, or at least 90% complementary to the SPN sequence, or least 80% complementary to the SPN sequence. In another embodiment, the complementary sequence may have additional polyA nucleotides. The short complementary sequence can easily detach from the corresponding SPN, in particular when a target allergen protein competes and binds to the SPN, enabling a highly sensitive detection assay.

In some aspects, the complementary sequence is labeled with a detection signal moiety e.g., a fluorophore, at either the 5′end or 3′end of the sequence. As non-limiting examples, the fluorophore may be selected from Alex Fluor @ fluorophores (such as Alex 514, Alex 532, Alex 546, Alex 555, Alex 568, Alex 594, Alex 610, Alex 633, Alex 635, Alex 647, Alex 660, Alex 680, Alexa 700, Alex 750, Alex 800, Alex 610-R-phycoerythrin (R-PE), Alex 647-R-phycoerythrin (R-PE), Alex 680-R-phycoerythrin (R-PE), and Alex 680-Allophycocyanin (APC)), Allophycocyanin (APC) and its derivatives, Cy fluorophores (e.g., Cy3.5, Cy3-FITC, CY5, CY 5.5, CY7, CY7-APC, CY5.5-APC), Qdots, TRITC, R-PE, Tamara, Rhodamine Red-X, Rox, TruRed, SYPRO red, BODIPY TR, Propidium iodide and Texas red. In some examples, the fluorophore is Alex 647, Cy5, Cy3-FITC or Texas red.

Detection Agents

Aptamers, signaling polynucleotides (SPNs) and SPN-complement complexes can be used as detection agents in a variety of allergen detection assays, biosensors, detection systems and devices as disclosed in the prior art, either as free agents or conjugates to other support substances. For example, aptamers, SPNs and SPN-complement complexes of the present invention may be used as surface bound affinity molecules that bind the surfaces of solid substrates. The solid surface may be a three-dimensional surface such as micro-spheres (e.g., magnetic beads/particles), or a two-dimensional surface such as the glass or silicon surface.

In one embodiment, aptamers, SPNs and SPN-complement complexes of the present invention are immobilized on the surface of magnetic particles to form functionalized magnetic particles which can capture a target analyte (e.g., allergen) in a fluid sample; the particles will be suitable for magnetic manipulations in a detection assay and method.

In some aspects, aptamers, SPNs and SPN-complement complexes of the present invention may be covalently immobilized on the surface of magnetic particles. In some aspects, SPNs may be covalently immobilized on the surface of magnetic particles through an amine (—NH2) group, or a thiol group (—SH) at one end the SPN sequence. In other aspects, complementary sequence of SPNs may be covalently immobilized on the surface of magnetic particles, from which the SPNs are attached to the particles. Concentrations of SPNs, complementary sequences and magnetic particles are optimized for the most effective binding to each other. In some aspects, SPNs and their complementary sequences may be at a ratio of 1:5, or at a ratio of 1:4, or at a ratio of 1:3, or at a ratio of 1:2.

In another embodiment, aptamers, SPNs and SPN-complement complexes of the present invention may be attached to a two-dimensional solid surface; said two dimensional solid surface may be a glass surface or the surface of a silicon chip. Such surfaces printed/coated with aptamers, SPNs, complements and/or SPN-complement complexes of the present invention may be used as biosensing platforms for a variety of assays and applications.

In some embodiments, detection agents of the present invention may be labeled with a fluorescent marker which generates detectable fluorescent signals. Either the SPN or its complementary sequence may be labeled with a fluorophore. In some aspects, the fluorophore is added to one end of the complement sequence, either the 5′end or 3′end, as illustrated in FIGS. 4A, 4B and 4C, and FIG. 5A. In other aspects, One end of the SPN may be labeled with a fluorophore, as shown in FIG. 5B. FIG. 6A and FIG. 6B. As non-limiting examples, the fluorophore may be selected from, Alex Fluor®, fluorophores (such as Alex 514, Alex 532, Alex 546, Alex 555, Alex 568, Alex 594, Alex 610, Alex 633, Alex 635, Alex 647, Alex 660, Alex 680, Alexa 700, Alex 750, Alex 800, Alex 610-R-phycoerythrin (R-PE), Alex 647-R-phycoerythrin (R-PE), Alex 680-R-phycoerythrin (R-PE), and Alex 680-Allophycocyanin (APC)), Allophycocyanin (APC) and its derivatives, Cy fluorophores (e.g., Cy3.5, Cy3-FITC, CY5, CY 5.5, CY7, CY7-APC, CY5.5-APC), Qdots, TRITC, R-PE, Tamara, Rhodamine Red-X, Rox, TruRed, SYPRO red, BODIPY TR, Propidium iodide and Texas red. In some examples, the fluorophore is Alex 647, Cy5, CY3-FITC or Texas red.

1. Magnetic Particles/Beads

Magnetic particles have several advantages that make them attractive substrates for use as signal transducers, including their biological inertness, physical stability, and the absence of competing magnetic signals in biological materials (Gijs et al., Chem Rev. 2010; Vol 110(3), 1518-1563).

Magnetic particles may be any particle materials that can be separated by magnetic forces. Magnetic particles for bioresearch may consist of one or more magnetic cores with a coating matrix of polymers, silica or hydroxylapatite with terminal functionalized groups. The magnetic core generally consists either of magnetite (Fe₃O₄) or maghemite (γ-Fe₂O₃) with superparamagnetic or ferromagnetic properties. For example, magnetic cores can be made with magnetic ferrites, such as cobalt ferrite or manganese ferrite. Such magnetic micro- or nanospheres can be separated easily and quickly by magnetic forces and can be used together with bioaffine ligands, e.g. antibodies or aptamers with a high affinity to the target.

In one example, magnetic particles or beads may be synthesized by dispersing ferrite crystals in a suspension of styrene, divinylbenzene monomers and polymerizing the cocktails into microparticles. In another example, magnetic particles/beads may be synthesized by coating one or more layers of magnetite onto a polystyrene core. Multiple layers of magnetite may increase the speed by which the particle/bead responds to a magnetic field. The synthesized microparticles are encapsulated with inert polymers such as polystyrene to prevent the iron from interfering with any subsequent biochemical reactions. Polystyrene magnetic beads can be used for with both carboxylic acid and amine surface chemistries.

Additional polymers that may be used to prepare magnetic particles/beads include, but are not limited to, alginate, dextran, polyacrylamide, polycaprolactone, polyethylenimine (PEI), polyisopropene, poly(2-cinnamoylethyl methacrylate), poly(acetoacetoxyethyl methacrylate), poly(dimethylsiloxane), poly(ethylene glycol)-poly(aspartic acid) (PEG-PAsp), poly(ethylene oxide), poly(glutamic acid), poly(glycidyl methacrylate), poly(lactide), poly(lactide-co-glycolide), poly(1-lactic acid), poly(l-lactide-co-glycolide), poly(methyl methacrylate-divinylbenzene), poly(N-isopropyl acrylamide) (PNIPA), poly(N-vinylcaprolactam), poly(styrene-acetoacetoxyethylmethacrylate) (PSAAEM), poly(styrene-butyl acrylate-methacrylic acid), poly(styrene-co-acrylamide), poly(styrene-co-acrylic acid), poly(styrene-co-butyl acrylate), poly(styrene-divinylbenzene-glycidyl methacrylate), poly(styrene-methacrylic acidacrylamide), poly(tert-butyl acrylate), poly(vinyl alcohol) (PVA), and any combinations thereof.

Magnetic particles may also be coated with streptavidin, maleimide, amino groups or carboxyl groups to optimize aptamer affinity. DNA specificity and non-specific adsorption of DNAs on their surfaces.

In addition to chemical modifications on the surface, magnetic particles may be in a size with maximal efficiency and affinity to the conjugated nucleic acids. As used herein, the particle size (or particle diameter) is given as a hydrodynamic diameter, which includes the core diameter and two times the diameter of the cover matrix. The size of the particle determines the surface area available for the attachment of functional groups. Increasing the size reduces the surface-to-volume ratio therefore resulting in a decrease of the available surface area per volume for modification, but speeding up its response in a magnetic field which makes it easier to be manipulated. In some examples, magnetic particles may be in a wide range of average particle sizes, from 100 nm to 5.0 μm in the diameter, having optimized parameters such as sedimentation rate, available binding sites, and magnetic volume. In some aspects, the average magnetic particle size may be from 100 nm to 800 nm, or from 200 nm to 500 nm, or from 0.1 μm to 3.0 μm, the size may be 100 nm, 125 nm, 150 nm, 200 nm, 250 nm, 300 nm, 350 nm, 400 nm, 450 nm, 500 nm, 550 nm, 600 nm, 700 nm, 800 nm, 900 nm, 0.2 μm, 0.3 μm, 0.4 μm, 0.5 μm, 0.6 μm, 0.7 μm, 0.8 μm, 0.9 μm, 1.0 μm, 1.5 μm, 2.0 μm, 2.5 μm, 3.0 μm, 3.5 μm, 4.0 μm, 4.5 μm, or 5.0 μm.

In some cases, magnetic particles may have an irregular or rough surface. As curvature can introduce additional surface area, irregular or rough surface increases the overall surface area available for the attachment of nucleic acid molecules.

As non-limiting examples, magnetic particles may be fluidMAG particles (which is hydrophilic). SiMAG particles (which are magnetic silica beads with superparamagnetic or ferromagnetic properties and possess either a highly porous or a non-porous silica surface), mHPA-particles (which are non-spherical with hydroxylapatite coated ferromagnetic particles with a diameter of 2 μm, consisting of calcium phosphate), ZeoliteMAG (which are magnetic zeolite particles, which consist of a superparamagnetic iron oxide core and a high-porous aluminosilicate matrix), beadMAG-particles (which are magnetic particles with a diameter of 1 μm, covered with a hydrophilic matrix of crosslinked starch with terminal cation-exchange phosphate groups), and magTosyl-magnetic beads or other appropriately derived magnetic beads for nucleic acid conjugations. In some embodiments, polystyrene magnetic particles may be used. The magnetic particles may also be sepharose magnetic microbeads and agarose magnetic microbeads.

In some embodiments, magnetic particles, in the absence of a magnetic field, may exhibit no net magnetization, but within a magnetic field, the magnetic moments of the bead align with the field, making the beads magnetic.

2. Other Solid Substrates

Aptamers, SPNs and/or SPN-complement complexes may be attached to any two-dimensional solid surfaces such as microtiter plates, silicon chips and printed glass surfaces (e.g. epoxy saline-derived glass surfaces). Other examples of suitable solid substrates (also called solid supports) may include, but are not limited to, those made of silica or silica-based materials, functionalized glass, modified silicon, inorganic glasses, plastics, resins, polysaccharides, carbon, metals, nylon, natural fibers such as silk, wool and cotton, and polymers. Solid substrates may have any useful form including thin films or membranes, beads, microwell plates, dishes, slides, fibers, woven fibers, shaped polymers, particles, chips, wafers and microparticles. Solid substrates may be porous or non-porous.

In some embodiments, the two-dimensional surface may be a surface of a glass or silicon slide. Glass is a readily available and inexpensive support medium that has low intrinsic fluorescence. The surface of the glass or silicon slide may be modified or unmodified, although most attachment protocols involve chemically modifying the glass surface to facilitate attachment of the oligonucleotides. Glass has a relatively homogeneous chemical surface whose properties have been well studied and is amenable to chemical modification using very versatile and well developed silanization chemistry. In certain embodiments, the surface of the glass or silicon slide is unmodified. For example, silianized oligonucleotides can be covalently linked to an unmodified glass surface (Kumar et al., Nucleic Acids Res. 2000 Jul. 15; 28(14): e71).

In certain embodiments, the surface of glass or silicon is chemically modified. Glass surface can be treated with an amino silane to have a uniform layer of primary amines or epoxides. In one example, oligonucleotides modified with an NH2 group can be immobilized onto epoxy silane-derivatized or isothiocyanate coated glass slides. In another example, succinylated oligonucleotides can be coupled to aminophenyl- or aminopropyl-derivitized glass slides by peptide bonds. In yet another example, disulfide-modified oligonucleotides can be immobilized onto a mercaptosilanized glass support by a thiol/disulfide exchange reactions or through chemical cross linkers.

In some embodiments, graphene oxide (GO) may be used as signal transducers in replacement of magnetic particles. Graphene oxide (GO) is a single-atom-thick two-dimensional carbon nanomaterial widely used in biosensor applications due to its unique optical electronic, thermal, and long-lasting biocompatibility properties (also known as graphene oxide nanosheet and graphene nanosheet). Most importantly. GO has superior fluorescence quenching capacity and unique adsorption characteristics for biomolecules. The quenching capacity is due to self-assembly of graphene oxide through specific π-π interactions.

GO is graphite oxidized to intersperse the carbon layers with oxygen molecules, and then reduced to separate the carbon layers completely into individual or few layer graphene. GO can be synthesized by the oxidative treatment of graphite by one of the principle methods developed by Brodie, Hummers or Staudenmeir in the art. A number of modified methods are also available (Paulchamy, et al., J Nanomed Nanotechnol, 2015, 6:1. doi: 10.4172/2157-7439.1000253; Jasim, et al., 2D Mater. 2016, 3, 014006. doi: 10.1088/2053-1583/3/1/014006; and Shahriary and Athawale, Int. J. Renew. Energy Environ. Eng, 2014, Vol. 02 (01): 58-63; the contents of each of which are incorporated herein by reference in their entirety.)

In some embodiments, SPNs and/or SPN-complement complexes may be attached onto the GO surface through physical adsorption. In this aspect, SPNs or SPN-complement complexes may be labeled with Qdots. When Qdots-aptamer conjugates are attached onto GO, the fluorescence signal is quenched due to non-radioactive electronic excitation energy transfer between the fluorophore and GO. In the presence of a target molecule, the interaction between the target molecule and the aptamer is stronger than that between the aptamer and GO, resulting in the release of the aptamer and therefore recovery of the fluorescence signal.

3. Conjugation Chemistry and Methods

Aptamers, SPNs and SPN complementary sequences can be conjugated to magnetic particles by any method known in the art which are used to conjugate nucleic acid molecules to solid surfaces. The methods may be irreversible immobilization methods or reversible immobilization methods. As non-limiting examples, methods may include biotin-streptavidin system, and EDC mediated carboxyl-to-amine crosslinking (e.g., covalent binding of amino-modified aptamer (SPNs) to carboxyl-functionalized magnetic particles), Aldehyde-activated sugars; and cross linkers used to modify nucleic acids and solid surfaces for conjugations (Scientific, Thermo (2012), Crosslinking Technical Handbook, Thermo Fisher Scientific Inc., Waltham, USA).

In some embodiments, the short complementary sequences may be bound to a solid surface. In other embodiments, the SPN may be bound to a solid surface.

In some embodiments, nucleic acid molecules (e.g. aptamers, SPNs, and SPN complement) of the present invention are conjugated to the surface of magnetic particles at one end, e.g. the 5′ end or 3′end (e.g., as shown in FIGS. 4A, 4B, 4C and FIG. 5B). Nucleic acids can be covalently attached to magnetic particles/beads by methods based on the formation of covalent bonds. Carboxyl and amino groups are the most common reactive groups for attaching ligands to surfaces. Examples of the reactive groups that can be incorporated on the micro-bead surface and/or the termini of ligands for covalent coupling may include but are not limited to, carboxylic acid (—COOH). Primary aliphatic amine (—RNH₂), Aromatic amine (—ArNH₂), Chloromethyl (vinyl benzyl chloride) (—ArCH₂CL), Amide (—CONH₂), Hydrazide (—CONHNH₂), Aldehyde (—CHO), Hydroxyl (—OH), Thiol (—SH) and Epoxy (—COC—).

In some aspects, an amino group may be attached to the 5′ or 3′ end of the nucleic acid sequence. Various amino modifiers such as β-cyanoethyl phosphoramidites can be added to the 5′ end of a nucleic acid molecule. 5′ amino modifiers can be simple amino groups with a six or twelve carbon spacers, a Uni-Link amino modifier, or amino modified thymidine or cytosine. Amino modifiers that can be added to the 3′ end of a nucleic acid molecule (e.g., SPN), may be CPGs. In one example, a primary amine (—NH2) modifier may be placed to the 5′end, or 3′end of a nucleic acid molecule (e.g., SPN), or internally using an amino-C or amino-T modified base. The amino-modified nucleic acid molecules may be attached to magnetic particles using an acylating reagent, including but not limiting to Carbodiimide (EDC), Isothiocyanate, Sulfonyl chloride, and Succinimidyl esters (NHS-ester). In one aspect, amine-modified nucleic acids can then be reacted with carboxylate-modified microparticles with carbodiimide mediated acylation in a one-step coupling, which is fast and inexpensive. In addition, Acylation of a carboxyl group generates a stable carbonyl amide. One example of carbodiimide may be water soluble EDAC (1-ethyl-3-(3-dimethylaminopropyl) carbodiimide hydrochloride). Alternatively, amine-modified nucleic acids may be attached to magnetic particles with Isothiocyanates, which form thioureas linkage upon reaction with amines. The thioureas linkage is relatively stable.

In other aspects, a thiol group (e.g., thiol meliamide) is attached to the 5′ or 3′ end of a nucleic acid molecule (e.g., a SPN). The thiol (—SH) modifier enables covalent attachment of a nucleic acid molecule to a variety of substrates including magnetic particles, via disulfide bond (—S—S—) or maleimide linkages. The incorporation of a thiol group at the 5′ end of a nucleic acid molecule may be achieved with S-trityl-6-mercaptohexyl derivatives. The 3′-thiol modifier C3 S—S CPG may be used to introduce a thiol group to the 3′-end of a nucleic acid molecule.

In one particular example, a short polyA sequence (e.g., 5 nt) may be added at the end of the SPN or the complementary sequence. The polyA tail then is modified with a thiol group. The reaction between thiol-DNA and carboxylated magnetic beads is mediated by maleimide which is attached to Poly(ethylene glycol) (PEG) polymer coated solid substrates. It is believed that the distance created by the addition of polyA residues and PEG, increases the binding between the bead and DNA and the stability of DNA on the surface of magnetic particles. At the same time, PEG linkers may reduce non-specific binding.

In some examples, cross linkers may be used to attach thiol, or amine-modified nucleic acids to the surface of magnetic beads. As used herein, the term “cross-linker” means a functional chemical group that covalently binds two distinct chemical groups and generates a physical space between the two entities which provides greater accessibility and or freedom to each of the linked biomolecules. A number of cross-linkers may be used to develop covalent attachment of thiol or amine modified nucleic acids to solid surfaces, such as succinimidyl 4-[maleimidophenyl]butyrate (SMPB).

Magnetic particles may also be coated with streptavidin, maleimide, other amino groups or carboxyl groups to optimize aptamer affinity, DNA specificity and non-specific adsorption of DNAs on their surfaces.

In one example, the coupling of nucleic acids and surfaces may be through the binding of biotin-labeled nucleic acids to streptavidin-coated beads. The biotin-streptavidin linkage can tether nucleic acid molecules to the solid surface (e.g. magnetic particles). In another example, nucleic acid molecules and/or solid substrates may be coupled by ethanolamine and heterobifunctional poly (ethylene glycol) (PEG) linkers, which allow the covalent binding of nucleic acid molecules to the solid substrates (e.g. magnetic particles and glass slides). Accordingly, magnetic beads (or other solid substrates such as glass slides) are coated with PEG polymers. PEG polymers coated magnetic particles are further modified to add an active agent such as a carboxyl group, an amine group, a maleimide and a neutravidin. The PEG linkers will change the surface force, nucleic acid stability and non-specific binding. A detailed protocol is described by Janissen et al (Nucleic acid Research, 2014, 42(18): e137; the contents of which are incorporated herein by reference in its entirety).

In addition to chemical modifications on the surface, magnetic beads may be in a size with maximal efficiency and affinity to the linked nucleic acids. Magnetic particles or beads may be synthesized by dispersing ferrite crystals in a suspension of styrene, divinylbenzene monomers and polymerizing the cocktails into microparticles. (Polystyrene magnetic beads can be used for with both carboxylic acid and amine surface chemistries.)

In some aspects, acid treated magnetic particles containing hydroxyl (OH) groups on the surface can be used to conjugate ligands including aptamers as disclosed in U.S. Patent application publication No.: US2014/0206822, the contents of which are incorporated herein by reference in its entirety.

In further another example, molecular spacers may be used to mediate the coupling between aptamers and magnetic particles. The method can avoid interaction between the solid surface and the aptamer conformation.

Aptamers, SPNs and SPN-complement complexes may also be conjugated to a glass surface or other two-dimensional surfaces through chemical modifications known in the art. In some aspects, the solid surface treatment may include, but is not limited to epoxy silane coated glass, isothiocyanate coated glass, aminophenyl or aminopropyl-derivatized glass, mercaptosilanized glass support, aldehyde or epoxide treatment. Amine (NH2), succinylation, disulfide and hydrazide (e.g., I-Linker™) may be used to modify oligonucleotide to facilitate the attachment of DNA to different surfaces.

A two-dimensional surface may be prepared by treating the glass surface with an amino silane which will result in a uniform layer of primary amine or epoxides. Parameters that affect the binding of oligonucleotides to the surface may be optimized to achieve the greatest specificity and DNA density. A high surface coverage of the oligonucleotide may generate a higher signaling due to higher hybridization between SPNs and their complementary sequences. The fluorescence background, chemical stability, complexity, amenability to chemical modification, surface area, loading capacity, and the degree of non-specific binding of detect molecule are adjusted for choosing appropriate surface support and conjugating chemistry.

For example, to increase the loading capacity of oligonucleotides on the planar surface structures of glasses, acrylamide gels can be applied to glasses to construct a—three-dimensional surface which will increase the surface area for DNA attachment.

4. In Situ Oligonucleotide Synthesis on Solid Support

In addition to attaching a synthesized aptamer, SPN or a SPN-complementary sequence to a solid support, nucleic acid molecules (e.g. aptamers, SPNs, and SPN complementary sequence) of the present invention can also be synthesized in situ on a solid support such as on magnetic particles, glass slides, wafers, microwell plates and silicon chips. Compared to the conventional method which requires the oligonucleotides to be pre-synthesized with specific end modifications to fit the surface attachment chemistry, this method can streamline the process of synthetic preparation by eliminating these steps.

The nucleic acid molecule can be synthesized by (a) covalently attaching one or more phosphoramidite linkers to the functional groups on the solid substrate to produce a derivatized support. (b) reacting the derivatized support with a nucleoside phosphoramidite corresponding to the first nucleotide of desired nucleotide sequence, and (c) adding nucleoside phosphoramidite stepwise until the entire oligonucleotide is assembled. Nucleoside phosphoramidites are preferred because naturally occurring nucleotides and their phosphodiester analogs are insufficiently reactive for an expeditious synthesis of oligonucleotides in high yields. Non-nucleoside phosphoramidites may be used to produce modified oligonucleotides.

External forces may be used to immobilize the solid substance during synthesis. For example, nucleic acid molecules may be synthesized on paramagnetic beads using the methods described in U.S. patent application Ser. No. 14/280,609 and Jensen et al., J Biotechnol, 2013, Sep. 20; 167(4); the contents of which are hereby incorporated by reference. The approach uses an external magnet to hold the paramagnetic beads in place during synthesis.

The nucleic acid synthesis can be performed in either the 5′ to 3′ direction or the 3′ to 5′ direction by suitable choice of nucleoside phosphoramidite reagents. For example, 3′-[(2-cyanoethyl)-(N,N-diisopropyl)]-phosphoramidites can be used for synthesis in the 3′ to 5′ direction. Alternatively, 5′-[(2-cyanoethyl)-(N,N-diisopropyl)]-phosphoramidites (Glen Research) can be used for synthesis in the 5′ to 3′ direction.

In certain embodiments, the substrate functional group used for attachment of the linker is a hydroxyl group or an amino group. For example, a hydroxylated substrate, such as hydroxylated polystyrene may be used for attachment of the linker. Phosphoramidite linkers are used to reduce steric hindrance associated with neighboring base-base interactions. In certain embodiments, the phosphoramidite linker is between 30 and 60 atoms in length. Exemplary phosphoramidite linkers include those disclosed in U.S. patent application Ser. No. 14/280,609; the contents of which are incorporated herein in its entirety.

5. Optimizing Oligonucleotide Synthesis on a Solid Support

In some embodiments, the short oligonucleotide sequences directly synthesized on a solid surface may be further optimized to fit the purpose of detection agents. In accordance with the present invention, a short sequence that is directly synthesized on a solid support (e.g., the surface of magnetic beads) will form a complex with the aptamer. The short oligonucleotide is complementary to one end of the aptamer sequence. The aptamer-complement complexes linked on the solid support are then used as detection agents. To fulfill this purpose, short complement sequences attached on a solid surface may meet the following features: (1) the oligonucleotides cannot be cleaved off from the surface following synthesis; (2) the oligonucleotides are being held away from the surface to allow hybridization with the complementary sequence on the aptamer to form aptamer-complement complexes; and (3) only low to moderate density of the complementary oligonucleotides are synthesized on the solid surface.

As described above, a standard 3′ to 5′ phosphoramidite chemical reaction may be used to for oligonucleotide synthesis. Automated synthesizers may be used to synthesize the short oligonucleotides using magnetic beads as supports. In one example, highly cross-linked polystyrene (PS) beads with proper particle sizes and good moisture exclusion properties may be used for efficient oligonucleotide synthesis. The polystyrene polymer may further bind together with magnetic particles (e.g., Fe3O4 particles) to form the solid support for direct oligonucleotide synthesis.

To stabilize synthesized oligonucleotide sequences on beads, non-cleavable stable linkers may be used for oligonucleotide synthesis. A non-cleavable linker is a chemical moiety immobilized on a solid support and not substantially cleaved under synthesis conditions (e.g., deprotection conditions). The linker may be covalently bound to a solid support (e.g., functionalized glass and magnetic beads).

Exemplary stable linkers may include, but are not limited to, amino linkers such as siloxane linkers, linkers containing alkyl groups such as —(OCH₂CH₂)_(n)— (n=1-20), —(CH₂)_(m)—C(O)NH—(CH₂)_(n)— and —(OCH₂CH₂)_(m)—C(O)NH—(OCH₂CH₂H₂)_(n)— (m and n can be the same or different and m and n are from about 1 to about 20), linkers containing amide groups like —R₁—C(O)NH—R₂—, monomethoxytrityl (MMT)-protected amino linker, monomethoxytrityl (MMT)-protected amino linker, trifluoroacetyl (TFA)-protected pentyl (C5) amino linker, and trifluoroacetyl (TFA)-protected hexyl (C6) amino linker. In some embodiments, the linker may be a complex linker comprising more than one functional group. Exemplary complex linkers may include those discussed in U.S. Pat. Nos. 7,553,958; 8,053,187; and 9,303,055; the contents of each of which are incorporated herein by reference in their entirety. Other non-cleavable linkers to solid supports may also include these disclosed in U.S. Pat. Nos. 8,569,515; and 8,853,132, the contents of each of which are incorporated herein by reference in their entirety.

In other embodiments, a spacer may be used to hold synthesized oligonucleotides away from the beads, therefore allow the short oligonucleotides to bind effectively to its complement on the end of the aptamer. As used herein, the term “spacer” refers to a chemical group connected to a linker that is used to extend the length of the linker moiety and as a site for initiating synthesis of a polymer chain. Examples of spacer include, but are not limited to, ethyleneglycol polymer, alkyl, oligonucleotides, peptides, and peptditomimetics. In other aspects, the spacer may be an anchor group that is attached to one end of the linker. The anchor group may be served as the site of oligonucleotide synthesis. At the end of oligonucleotide synthesis, a 5′DMT (4.4′-dimethoxytrityl) protecting group may be added to the last nucleoside, the role of which is to prevent interaction with the solid supports and between oligonucleotide polymers.

In some embodiments, low to moderate density of short oligonucleotides may be synthesized on the beads. The controlled loading allows for independent short oligonucleotides that have space to interact with the complementary sequence on the aptamer. The density of aptamer-complement complexes on the solid support may further be optimized to provide adequate signals when the conjugates are used in a detection assay.

In some embodiments, solid supports (e.g., magnetic beads and functionalized glasses) with synthesized oligonucleotides may be separated from the reaction suspension. For example, Magnet force may be used to pull down the beads from the reaction suspension. Separated beads are then read for fluorescent signals.

Target Allergens

Compositions, SPNs, SPN-complement complexes, magnetic particle conjugates and detection agents of the present invention may work as ligands for any target analyte. As stated below, the target analyte may be an allergen protein or variants thereof. In some embodiments, compositions, SPNs. SPN-complement complexes, magnetic particle conjugates and detection agents of the present invention may be designed to bind or associate with allergen proteins or other biomolecules which themselves associated with the allergen.

As used herein, the term “allergen” refers to a substance that can cause allergic reaction. An allergen is then a type of antigen that triggers an abnormally vigorous immune response in body.

Allergens include those from food products, the environment such as pollen, or animals such as a domestic pet dander. Food allergens include, but are not limited to proteins in legumes such as peanuts, peas, lentils and beans, tree nuts, wheat, milk, fish, egg white and sea food. Other allergens may be from the environment such as pollens, other animals (e.g., pet), pathogens and medicines. A comprehensive list of allergenic proteins from various sources is discussed below.

In some embodiments, allergens are food allergens. Examples of allergenic proteins associated with food include, but are not limited to, Brine shrimp (Art fr 5), Crab (Cha f 1), North Sea Shrimp (Cra c 1. Cra c 2, Cra c 4, Cra c 5, Cra c 6, Cra c 8), American lobster (Hom a 1, Hom a 3, Hom a 6), white shrimp (Lit v 1, Lit v 2, Lit v 3, Lit v4), giant freshwater prawn (Mac r 1), shrimp (Met e 1, Pen a 1, Pen i 1), northern shrimp (Pan b 1), spiny lobster (Pan s 1), black tiger shrimp (Pen m 1, Pen m 2, Pen m 3, Pen m 4, Pen m 6), narrow-clawed crayfish (Pon i 4, Pon i 7), blue swimmer crab (Por p 1), domestic cattle (Bos d 4, Bos d 5, Bos d 6, Bos d 7, Bos d 8, Bos d 9, Bos d 10, Bos d 11, Bos d 12), Atlantic herring (Clu h 1), common carp (Cyp c 1), Baltic cod (Gad c 1). Atlantic cod (Gad m 1, Gad m 2, Gad m 3), cod (Gad c 1), chicken (Gal d 1, Gal d 2, Gal d 3. Gal d 4, Gal d 5), Barramunda (Lat c 1), Lepidorhombus whiffiagonis (Lep w 1), chum salmon (One k 5), Atlantic salmon (Sal s 1, Sal s 2, Sal s 3) rainbow trout (One m 1), Mozambique tilapia (Ore m 4), edible frog (Ran e 1, Ran e 2), pacific pilchard (Sar sa 1), ocean perch (Seb m 1), yellowfin tuna (Thu a 1, Thu a 2, Thu a 3), swordfish (Xip g 1), abalone (Hal m 1), brown garden snail (Hel as 1), Squid (Tod p 1), pineapple (Ana c 1, Ana c 2), asparagus (Aspa o 1), barley (Hor v 12, Hor v 15, Hor v 16, Hor v 17, Hor v 20, Hor v 21), banana (Mus a 1, Mus a 2, Mus a 3, Mus a 4, Mus a 5), banana (Musxp1), rice (Ory s 12), rye (Sec c 20), wheat (Tri a 12, Tri a 14, Tri a 18, Tri a 19, Tri a 25, Tri a 26, Tri a 36, Tri a 37), maize (corn) (Zea m 14, Zea m 25), kiwi fruit (Act c1, Act c 2, Act c 5, Act c 8, Act c 10, Act d 1, Act d 2, Act d 3, Act d 4, Act d 5, Act d 6, Act d 7, Act d 8, Act d 9, Act d 10, Act d 1), cashew (Ana o 1, Ana o 2. Ana o 3), celery (Api g 1, Api g 2, Api g 3, Api g 4, Api g 5, Api g 6), peanut (Ara h 1, Ara h 2, Ara h 3, Ara h 4, Ara h 5, Ara h 6, Ara h 7, Ara h 8, Ara h 9, Ara h 10, Ara h 11, Ara h 12, Ara h 13), brazil nut (Ber e 1, Ber e 2), oriental mustard (Bra j 1), rapeseed (Bra n 1), cabbage (Bra o 3), turnip (Bra r 1, Bra r 2), bell pepper (Cap a 1w, Cap a 2), pecan (Car i 1, Car i 4), chestnut (Cas s 1, Cas s 5, Cas s 8, Cas s 9), lemon (Cit I 3), tangerine (Cit r 3), sweet orange (Cit s 1, Cit s 2, Cit s 3), Hazel (Cor a 1, Cor a 2, Cor a 8, Cor a 9, Cor a 11, Cor a 12, Cor a 13, Cor a 14), muskmelon (Cuc m 1, Cuc m 2, Cuc m 3), carrot (Dau c 1, Dau c 4, Dau c 5), common buckwheat (Fag e 2, Fag e 3), tartarian buckwheat (Fag t 2), strawberry (Fra a 1, Fra a 3, Fra a 4), soybean (Gly m 1, Gly m 2, Gly m 3, Gly m 4, Gly m 5, Gly m 6, Gly m 7, Gly m 8), sunflower (Hel a1, Hel a 2, Hel a 3), black walnut (Jug n 1, Jug n 2), English walnut (Jug r 1, Jug r 2, Jug r 3, Jug r 4), Cultivated lettuce (Lac s 1), Lentil (Len c 1, Len c 2, Len c 3), litchi (Lit c 1), narrow-leaved blue lupin (Lup an 1), apple (Mal d 1, Mal d 2, Mal d 3, Mal d 4), Cassava (Man e 5), mulberry (Mor n 3), avocado (Pers a 1), green bean (Pha v 3), pistachio (Pis v 1, Pis v 2, Pis v 3, Pis v 4, Pis v 5), pea (Pis s 1, Pis s 2), apricot (Pru ar 1, Pru ar 3), sweet cherry (Pru av 1, Pru av 2, Pru av 3, Pru av 4), European plum (Pru d 3), almond (Pru du 3, Pru du 4, Pru du 5, Pru du 6), peach (Pru p 1, Pru p 2, Pru p 3, Pru p 4, Pru p 7), pomegranate (Pun g 1), pear (Pyr c 1, Pyr c 3, Pyr c 4, Pyr c 5), castor bean (Ric c 1), red raspberry (Rub i 1, Rub i 3), Sesame (Ses i 1, Ses i 2, Ses i 3, Ses i 4, Ses i 5, Ses i 6, Ses i 7), yellow mustard (Sin a 1, Sin a 2, Sin a 3, Sin a 4), tomato (Sola I 1, Sola I 2, Sola I 3, Sola I 4), potato (Sola t 1, Sola t 2, Sola t 3, Sola t 4), Mung bean (Vig r 1, Vig r 2, Vig r 3, Vig r 4, Vig r 5, Vig r 6), grape (Vit v 1), Chinese date (Ziz m 1), Anacardium occidentale (Ana o 1.0101, Ana o 1.0102), Apium graveolens (Api g 1.0101, Api g 1.0201), Daucus carota (Dau c1.0101, Dau c1.0102, Dau c1.0103, Dau c1.0104, Dau c1.0105, Dau c1.0201), Citrus sinensis (Cit s3.0101, Cit s3.0102), Glycine max (Gly m1.0101, Gly m1.0102, Gly m3.0101, Gly m3.0102), Lens culinaris (Len c1.0101, Len c1.0102, Len c1.0103), Pisum sativum (Pis s1.0101, Pis s1.0102), Lycopersicon sativum (Lye e2.0101, Lye e2.0102), Fragaria ananassa (Fra a3.0101, Fra a3.0102, Fra a3.0201, Fr a3.0202, Fra a3.0203, Fra a3.0204, Fra a3.0301), Malus domestica (Mal d1.0101, Mal d1.0102, Mal d1.0103, Mal d1.0104, Mal d1.0105, Mal d1.0106, Mal d1.0107, Mal d1.0108, Mal d1.0109, Mal d1.0201, Mal d1.0202, Mal d1.0203, Mal d1.0204, Mal d1.0205, Mal d1.0206, Mal d1.0207, Mal d1.0208, Mal d1.0301, Mal d1.0302, Mal d1.0303, Mal d1.0304, Mal d1.0401, Mal d1.0402, Mal d1.0403, Mal d3.0101w, Mal d3.0102w, Mal d3.0201w, Mal d3.0202w, Mal d3.0203w, Mal d4.0101, Mal d4.0102, Mal d4.0201, Mal d4.0202, Mal d4.0301, Mal d4.0302), Prunus avium (Pru av1.0101, Pru av1.0201, Pru av 1.0202, Pru av1.0203), and Prunus persica (Pru p4.0101, Pru p4.0201); and any variants thereof. The names of allergens associated with food are systematically named and listed according to IUIS Allergen Nomenclature Sub-Committee (see, International Union of Immunological Societies Allergen Nomenclature Sub-Committee, List of isoallergens and variants.)

In addition to food allergens, SPNs, magnetic particle conjugates and compositions of the present invention may detect airborne particulates/allergens and other environmental allergens. Samples that contain allergens may be obtained from plants (e.g. weeds, grasses, trees, pollens), animals (e.g., allergens found in the dander, urine, saliva, blood or other bodily fluid of mammals such as cat, dog, cow, pig, sheep, horse, rabbit, rat, guinea pig, mouse and gerbil), fungi/mold, insects (e.g., stinging insects such as bee, wasp, and hornet and chirnomidae (non-biting midges), as well as other insects such as the housefly, fruit fly, sheep blow fly, screw worm fly, grain weevil, silkworm, honeybee, non-biting midge larvae, bee moth larvae, mealworm, cockroach and larvae of Tenibrio molitor beetle; spiders and mites such as the house dust mite), rubbers (e.g. latex), metals, chemicals (e.g. drugs, protein detergent additives) and autoallergens and human autoallergens (e.g. Hom s 1, Hom s 2, Hom s 3, Hom s 4, Hom s 5) (see, Allergen Nomenclature: International Union of Immunological Societies Allergen Nomenclature Sub-Committee, List of allergens and Allergen Nomenclature: International Union of Immunological Societies Allergen Nomenclature Sub-Committee, List of isoallergens and variants).

Examples of allergenic proteins from plants that can be detected using the compositions of the present invention include, but are not limited to, ash (Fra e 1), Japanese cypress (Cha o1, Cha o 2), sugi (Cry j 1, Cry j 2), cypress (Cup a 1), common cypress (Cup s 1, Cup s 3), mountain cedar (Jun a 1, Jun a 2, Jun a 3, Jun s 1), prickly juniper (Jun o 4), eastern red cedar (Jun v 1, Jun v 3), sweet vernal grass (Ant o 1), saffron crocus (Cro s 1, Cro s 2), Bermuda grass (Cyn d 1, Cyn d 7, Cyn d 12, Cyn d 15, Cyn d 22w, Cyn d 23, Cyn d 24), orchard grass (Dac g 1, Dac g 2, Dac g 3, Dac g 4, Dac g 5), meadow fescue (Fes p 4), velvet grass (Hol I 1, Hol I 5), barley (Hor v 1, Hor v 5), rye grass (Lol p 1, Lol p 2, Lol p 3, Lol p 4, Lol p 11), bahia grass (Pas n 1), canary grass (Pha a 1, Pha a 5), timothy (Phl p 1, Phi p 2, Phi p 4, Phi p 5, Phi p 6, Phl p 7, Phl p 11, Phl p 12, Phi p 13), date palm (Pho d 2), Kentucky blue grass (Poa p 1, Poa p 5), rye (Sec c 1, Sec c 5, Sec c 38), Johnson grass (Sor h 1), wheat (Tri a 15, Tri a 21, Tri a 27, Tri a 28, Tri a29, Tri a30, Tri a 31, Tri a32, Tri a 33, Tri a 34, Tri a 35, Tri a 39), maize (Zea m 1, Zea m 12), alder (Aln g 1, Aln g 4), redroot pigweed (Ama r 2), short ragweed (Amb a 1, Amb a 2, Amb a 3, Amb a 4, Amb a 5, Amb a 6, Amb a 7, Amb a 8, Amb a 9, Amb a 10, Amb a 11), western ragweed (Amb p 5), giant ragweed (Amb t 5), mugwort (Art v 1, Art v 2, Art v 3, Art v 4, Art v 5, Art v 6), sugar beet (Beta v 1, beta v 2), European white birch (Bet v 1, Bet v 2, Bet v 3, Bet v 4, Bet v 6, Bet v 7), turnip (Bra r 5), hornbeam (Car b 1), chestnut (Cas s 1), rosy periwinkle (Cat r 1), lamb's-quarters, pigweed (Che a 1, Che a 2, Che a 3), Arabian coffee (Cof a 1, Cof a 2, Cof a 3), Hazel (Cor a 6, Cor a 10), Hazel nut (Cor a1.04, Cor a2, Cor a8), European beech (Fag s 1), ash (Fra e 1), sunflower (Hel a 1, Hel a 2), para rubber tree (Hev b 1, Hev b 2, Hev b 3, Hev b 4, Hev b 5, Hev b 6, Hev b 7, Hev b 8, Hev b 9, Hev b 10, Hev b 11, Hev b 12, Hev b 13, Hev b 14). Japanese hop (Hum j 1), privet (Lig v 1), Mercurialis annua (Mer a 1), olive (Ole e 1, Ole e 2, Ole e 3, Ole e 4, Ole e 5, Ole e 6, Ole e 7, Ole e 8, Ole e 9, Ole e 10, Ole e 11), European hophornbeam (Ost c 1), Parietaria judaica (Par j 1, Par j 2, Par j 3, Par j 4), Parietaria officinalis (Par o 1), Plantago lanceolata (Pal I 1), London plane tree (Pla a 1, Pla a 2, Pla a 3), Platanus orientalis (Pla or 1, Pla or 2, Pla or 3), white oak (Que a 1), Russian thistle (Sal k 1, Sal k 2, Sal k 3, Sal k 4, Sal k 5), tomato (Sola I 5), Lilac (Syr v 1, Syr v 5), Russian-thistle (Sal k 1), English plantain (Pla 11), Ambrosia artemisiifolia (Amb a8.0101, Amb a8.0102, Amb a9.0101, Amb a9.0102), Plantago lanceolata (Pla 11.0101, Pla 11.0102, Pla 11.0103), Parietaria judaica (Par j 3.0102), Cynodon dactylon (Cyn d1.0101, Cyn d1.0102, Cyn d1.0103, Cyn d1.0104, Cyn d1.0105, Cyn d1.0106, Cyn d1.0107, Cyn d1.0201, Cyn d1.0202, Cyn d1.0203, Cyn d1.0204), Holcus lanatus (Hol 11.0101, Hol 11.0102), Lolium perenne (Phl p1.0101, Phl p1.0102, Phl p4.0101, Phl p4.0201, Phl p5.0101, Phl p5.0102, Phl p5.0103, Phi p5.0104, Phl p5.0105, Phl p5.0106, Phl p5.0107, Phl p5.0108, Phl p5.0201, Phl p5.0202), Secale cereale (Sec c20.0101. Sec c20.0201), Betula Verrucosa (Bet v1.0101, Bet v1.0102, Bet v 1.0103, Bet v 1.0201, Bet v 1.0301, Bet v1.0401, Bet v 1.0402, Bet v 1.0501, Bet v 1.0601, Bet v 1.0602, Bet v1.0701, Bet v1.0801, Bet v1.0901, Bet v1.1001, Bet v1.1101, Bet v1.1201, Bet v 1.1301, Bet v1.1401, Bet v1.1402, Bet v1.1501, Bet v1.1502, Bet v1.1601, Bet v1.1701, Bet v 1.1801, Bet v1.1901, Bet v1.2001, Bet v1.2101, Bet v1.2201, Bet v1.2301, Bet v1.2401, Bet v 1.2501, Bet v1.2601, Bet v1.2701, Bet v1.2801, Bet v1.2901, Bet v1.3001, Bet v1.3101, Bet v 6.0101, Bet v6.0102), Carpinus betulus (Car b1.0101, Car b1.0102, Car b1.0103, Car b1.0104, Car b1.0105, Car b1.0106, Car b1.0106, Car b1.0106, Car b1.0106, Car b1.0107, Car b1.0107, Car b1.0108, Car b1.0201, Car b1.0301, Car b1.0302), Corylus avellana (Cor a1.0101, Cor a1.0102, Cor a1.0103, Cor a1.0104, Cor a1.0201, Cor a1.0301. Cor a1.0401, Cor a1.0402, Cor a1.0403, Cor a1.0404), Ligustrum vulgare (Syr v1.0101, Syr v1.0102, Syr v1.0103), Cryptomeria japonica (Cry j2.0101, Cry j2.0102), and Cupressus sempervirens (Cup s1.0101, Cup s1.0102, Cup s1.0103, Cup s1.0104, Cup s1.0105), and any variants thereof.

Lupin is an herbaceous plant of the leguminous family belonging to the genus Lupinus. In Europe, lupin flour and seeds are widely used in bread, cookies, pastry, pasta, sauces, as well as in beverages as a substitute for milk or soy, and in gluten-free foods. The International Union of Immunological Societies (IUIS) allergen nomenclature subcommittee recently designated β-conglutin as the Lup an 1 allergen. (Nadal, et al., (2012) PLoS one, 7(4): e35253), and more recently, a high-affinity 11-mer DNA aptamer against Lup an 1 (β-conglutin) was reported (Nadal, et al., (2013), Anal. Bioanal. Chem. 405:9343-9349).

Examples of allergenic proteins from mites that can be detected using the compositions of the present invention include, but are not limited to, mite (Blo t 1, Blo t 3. Blo t 4, Blo t 5, Blo t 6, Blo t 10, Blo t 11, Blo t 12, Blo t 13, Blo t 19, Blot t 21); American house dust mite (Der f 1, Der f 2, Der f 3, Der f 7, Der f 10, Der f 11, Der f 13, Der f 14, Der f 15, Der f 16, Der f 17, Der f 18, Der f 22, Der f 24); Dermatophagoides microceras (house dust mite) (Der m 1); European house dust mite (Der p 1, Der p 2, Der p 3, Der p 4, Der p 5, Der p 6, Der p 7, Der p 8, Der p 9, Der p 10, Der p 11, Der p 14, Der p 15, Der p 20, Der p 21, Der p 23); Euroglyphus maynei (House dust mite) (Eur m 2, Eur m 2, Eur m 3, Eur m 4, Eur m 14); storage mite (Aca s 13, Gly d 2, Lep d 2, Lep d 5, Lep d 7, Lep d 10, Lep d 13, Tyr p 2, Tyr p 3, Tyr p 10, Tyr p 13. Tyr p 24), Dermatophagoides farinae (Der f1.0101, Der f1.0102, Der f1.0103, Der f1.0104, Der f1.0105, Der f2.0101, Der f2.0102, Der f2.0103, Der f2.0104, Der f2.0105, Der f2.0106, Der f2.0107, Der f2.0108, Der f2.0109, Der f2.0110, Der f2.0111, Der f2.0112, Der f2.0113, Der f2.0114, Der f2.0115, Der f2.0116, Der f2.0117), Dermatophagoides pteronyssinus (Der p 1.0101, Der p 1.0102, Der p 1.0103, Der p 1.0104, Der p1.0105, Der p1.0106, Der p1.0107, Der p1.0108, Der p1.0109, Der p1.0110, Der p1.0111. Der p1.0112, Der p1.0113, Der p1.0114, Der p1.0115, Der p1.0116, Der p1.0117, Der p1.0118, Der p1.0119, Der p1.0120, Der p1.0121, Der p1.0122, Der p1.0123, Der p2.0101, Der p2.0102, Der p2.0103, Der p2.0104, Der p2.0105, Der p2.0106, Der p2.0107, Der p2.0108, Der p2.0109, Der p2.0110, Der p2.0111, Der p2.0112, Der p2.0113), Euroglyphus maynei (Eur m2.0101, Eur m2.0102), Lepidoglyphus destructor (Lep d2.0101, Lep d2.0101, Lep d2.0101, Lep d2.0102, Lep d2.0201, Lep d2.020) and Glycphagus domesticus (Gly d2.0101, Gly d2.0201); and any variants thereof.

Examples of allergenic proteins from animals that can be detected using the compositions of the present invention include, but are not limited to, domestic cattle (Bos d 2, Bos d 3, Bos d 4, Bos d 5, Bos d 6, Bos d 7, Bos d 8), dog (Can f 1, Can f 2, Can f3, Can f 4, Can f 5, Can f 6), domestic horse (Equ c 1, Equ c 2, Equ c 3, Equ c 4, Equ c 5), cat (Fel d 1, Fel d 2, Fel d 3, Fel d 4, Fel d 5w, Fel d 6w, Fel d 7, Fel d 8), mouse (Mus m 1), guinea pig (Cav p 1, Cav p 2, Cav p 3, Cav p 4, Cav p 6), rabbit (Ory c 1, Ory c 3, Ory c 4) rat (Rat n 1), Bos domesticus (Bos d 2.0101, Bos d 2.0102, Bos d 2.0103) and Equus caballus (Equ c2.0101, Equ c 2.0102); and any variants thereof

Examples of allergenic proteins from insects that can be detected using the compositions of the present invention include, but are not limited to, yellow fever mosquito (Aed a 1, Aed a 2, Aed a 3). Eastern hive bee (Api c 1), giant honeybee (Api d 1), honey bee (Api m 1, Api m 2, Api m 3, Api m 4, Api m 5, Api m 6, Api m 7, Api m 8, Api m 9, Api m 10, Api m 11, Api m 12), pigeon tick (Arg r 1), German cockroach (Bla g 1, Bla g 2, Bla g 3, Bla g 4, Bla g 5, Bla g 6, Bla g 7, Bla g 8, Bla g 11), bumble bee (Bom p 1, Bom p 4, Bom t 1, Bom t 4), silk moth (Bomb m 1), midge (Chi k 10, Chi t 1, Chi t 1.01, Chi t 2, Chit 2. 0101, Chi t 2. 0102, Chit 3, Chit 4, Chit 5, Chit 6, Chi t 6.01, Chit 7, Chi t 8, Chit 9), cat flea (Cte f 1, Cte f 2, Cte f 3), yellow hornet (Dol a 5), white face hornet (Dol m 1, Dol m 2, Dol m 5), biting midge (For t 1, For t 2), Savannah Tsetse fly (Glo m 5), Asian ladybeetle (Har a 1, Har a 2), silverfish (Lep s 1), booklouse (Lip b 1), Australian jumper ant (Myr p 1, Myr p 2, Myr p 3), American cockroach (Per a 1, Per a 3, Per a 6, Per a 7, Per a 9, Per a 10), Indian meal moth (Plo i 1, Plo i 2), wasp (Pol a 1, Pol a 2, Pol a 5, Pole 1, Pol e 4, Pol e 5, Pol f 5, Pol g 1, Pol g 5, Pol m 5, Poly p 1, Poly s 5, Ves vi 5), Mediterranean paper wasp (Pol d 1, Pol d 4, Pol d 5), tropical fire ant (Sol g 2, Sol g 3, Sol g 4), Solenopsis invicta (red imported fire ant) (Sol I 1, Sol I 2, Sol I 3, Sol I 4), black fire ant (Sol r 2, Sol r 3), Brazilian fire ant (Sol s 2, Sol s 3), horsefly (Tab y 1, Tab y 2, Tab y 5), pine processionary moth (Tha p 1, Tha p 2), California kissing bug (Tria p 1), European hornet (Vesp c 1, Vesp c 5), Vespa magnifica (hornet) (Vesp ma 2, Vesp ma 5), Vespa mandarinia (Giant asian hornet) (Vesp m1, Vesp m 5), yellow jacket (Ves f 5, Ves g 5, Ves m 1, Ves m 2, Ves m 5), Vespula germanica (yellow jacket) (Ves p 5), Vespula squamosa (Yellow jacket) (Ves s 1, Ve s s5), Vespula vulgaris (Yellow jacket) (Ves v 1, Ves v 2, Ves v 3, Ves v 4, Ves v 5, Ves v 6), Blattella germanica (Bla g 1.0101, Bla g 1.0102, Bla g 1.0103, Bla g 1.02, Bla g 6.0101, Bla g 6.0201, Bla g 6.0301), Periplaneta Americana (Per a1.0101, Per a1.0102, Per a1.0103, Per a1.0104, Per a1.02, Per a3.01, Per a3.0201, Per a3.0202, Per a3.0203, Per a7.0101, Per a7.0102), Vespa crabo (Ves pc 5.0101, Ves pc 5.0101), Vespa mandarina (Vesp m 1.01, Vesp m 1.02); and any variants thereof.

Examples of allergenic proteins from fungi/mold that can be detected using the signaling polynucleotides and assays of the present invention include, but are not limited to, Alternaria alternata (Alternaria rot fungus) (Alt a 1, Alt a 3, Alt a 4, Alt a 5, Alt a 6, Alt a 7, Alt a 8, Alt a 10, Alt a 12, Alt a 13), Aspergillus flavus (fungus) (Asp fl 13), Aspergillus fumigatus (fungus) (Asp f 1, Asp f 2, Asp f 3, Asp f 4, Asp f 5, Asp f 6, Asp f 7, Asp f 8, Asp f9, Asp f 10, Asp f 11, Asp f 12, Asp f 13, Asp f 15, Asp f 16, Asp f 17, Asp f 18, Asp f22, Asp f 23, Asp f 27, Asp f 28, Asp f 29, Asp f 34), Aspergillus niger (Asp n 14, Asp n 18, Asp n 25), Aspergillus oryzae (Asp o 13, Asp o 21), Aspergillus versicolor (Asp v 13), Candida albicans (Yeast) (Cand a 1, Cand a 3), Candida boidinii (Yeast) (Cand b 2), Cladosporium cladosporioides (Cla c 9, Cla c 14), Cladosporium herbarum (Cla h 2, Cla h 5, Cla h 6, Cla h 7, Cla h 8, Cla h 9, Cla h 10, Cla h 12), Curvularia lunata (Synonym: Cochliobolus lunatus) (Cur I 1, Cur I 2, Cur I 3, Cur I 4), Epicoccum purpurascens (Soil fungus) (Epi p 1), Fusarium culmorum (N.A.) (Fus c 1, Fus c 2). Fusarium proliferatum (Fus p 4), Penicillium brevicompactum (Pen b 13, Pen b 26), Penicillium chrysogenum (Pen ch 13, Pen ch 18, Pen ch 20, Pen ch 31, Pen ch 33, Pen ch 35), Penicillium citrinum (Pen c 3. Pen c 13, Pen c 19, Pen c 22, Pen c 24, Pen c 30. Pen c 32), Penicillium crustosum (Pen cr 26), Penicillium oxalicum (Pen o 18), Stachybotrys chartarum (Sta c 3), Trichophyton rubrum (Tri r 2, Tri r 4), Trichophyton tonsurans (Tri t 1, Tri t 4), Psilocybe cubensis (Psi c 1, Psi c 2), Shaggy cap (Cop c 1, Cop c 2, Cop c 3, Cop c 5, Cop c 7), Rhodotorula mucilaginosa (Rho m 1, Rho m 2), Malassezia furfur (Malaf2, Malaf3, Malaf4), Malassezia sympodialis (Malas1, Malas5, Malas6, Malas7, Malas8, Malas9, Malas10, Malas11, Malas12, Malas13) and Alternaria alternate (Alt a1.0101, Alt a1.0102); and any variants thereof.

Examples of additional allergens include, but are not limited to, Nematode (Ani s 1, Ani s 2, Ani s 3, Ani s 4), worm (Asc s 1), soft coral (Den n 1), rubber (Latex) (Hev b 1, Hev b 2, Hev b 3, Hev b 5, Hev b 6, Hev b 7, Hev b 8, Hev b 9, Hev b 10, Hev b 11, Hev b 12, Hev b 13), obeche (Trip s 1) and Heveabrasiliensis (Hev b6.01, Hev b6.0201, Hev b6.0202, Hev b6.03, Hev b8.0101, Hev b8.0102, Hev b8.0201, Hev b8.0202, Hev b8.0203, Hev b8.0204, Hev b10.0101, Hev b10.0102, Hev b10.0103, Hev b11.0101, Hev b11.0102); and any variants thereof.

Table 5 provides a list of non-limiting examples of allergenic proteins from various species. In the table, in addition to the species and allergen name, provided are the biochemical name of the allergenic protein and the unique identification numbers from GenBank or UniProt databases. In some embodiments, SPNs, magnetic particle conjugates and compositions of the present invention may be used to detect any of the allergenic proteins listed in Table 5, or any variant, fragment or antigenic portion thereof.

TABLE 5 Allergen proteins Food SEQ ID Species Allergen Allergen Biochemical name GenBank Uniprot NO Animalia Arthropoda Acarus siro (Storage Aca s 13 No Fatty acid-binding protein ABL09307.1 B0KZJ6 805 mite) Aedes aegypti (Yellow Aed a 1 No Apyrase AAC37218 P50635 806 fever mosquito) Aedes aegypti (Yellow Aed a 2 No Salivary D7 protein AAA29347 P18153 807 fever mosquito) Aedes aegypti (Yellow Aed a 3 No Undefined 30 kDa salivary AAB58417 O01949 808 fever mosquito) protein Aedes aegypti (Yellow Aed a 4 No α-glucosidase P13080 / 809 fever mosquito) Aedes aegypti (Yellow Aed a 5 No Sarcoplasmic Ca⁺ (EF- XP_001653462.1 Q16XK7 810 fever mosquito) hand) binding protein Aedes aegypti (Yellow Aed a 6 No Porin3 XP_001654143.1 Q1HR57 811 fever mosquito) Aedes aegypti (Yellow Aed a 7 No Undefined protein XP_001654291.1 Q16TN9 812 fever mosquito) Aedes aegypti (Yellow Aed a 8 No Heat Shock cognate ABF18258.1 Q1HR69 813 fever mosquito) protein-70 Aedes aegypti (Yellow Aed a No Tropomyosin XP_001655954.1 Q17H75 814 fever mosquito) 10.0101 Aedes aegypti (Yellow Aed a No Tropomyosin XP_001655948.1 Q17H80 815 fever mosquito) 10.0102 Aedes aegypti (Yellow Aed a 11 No Lysosomal aspartic XP_001657556.1 Q03168 816 fever mosquito) protease Apis cerana (Asiatic Api c 1 No Phospholipase A2 AAK09361 Q9BMK4 817 honey bee) Apis dorsata (Giant Api d 1 No Phospholipase A2 Q7M4I5 Q7M4I5 818 honeybee) Apis mellifera (Honey Api m 1 No Phospholipase A2 CAA34681 P00630 819 bee) Apis mellifera (Honey Api m 2 No Hyaluronidase AAA27730 Q08169 820 bee) Apis mellifera (Honey Api m 3 No Acid phosphatase AAY57281 Q4TUB9 821 bee) Apis mellifera (Honey Api m 4 No Melittin CAA26038 P01501 822 bee) Apis mellifera (Honey Api m 5 No Dipeptidylpeptidase IV NP_001119715 B2D0J4 823 bee) Apis mellifera (Honey Api m 6 No / NP_001035360 Q27SJ8 824 bee) Apis mellifera (Honey Api m 7 No CUB serine protease AAN02286 Q8MQS8 825 bee) Apis mellifera (Honey Api m 8 No Carboxylesterase VI ACB70231 B2D0J5 826 bee) Apis mellifera (Honey Api m 9 No Serine carboxypeptidase ACN71203 C9WMM5 827 bee) Apis mellifera (Honey Api m 10 No Icarapin variant 2, ABF21078 Q1HHN7 828 bee) carbohydrate-rich protein Apis mellifera (Honey Api m No Major royal jelly protein 8, NP_001011564 B3GM11 829 bee) 11.0101 variant 1 Apis mellifera (Honey Api m No Major royal jelly protein 8, AAY21180 Q4ZJX1 830 bee) 11.0201 variant 2 Apis mellifera (Honey Api m 12 No Vitellogenin CAD56944 Q868N5 831 bee) Archaeopotamobius Arc s 8 Yes Triosephosphate isomerase CAD29196 Q8T5G9 832 sibiriensis (Crustacean species decapod) Argas reflexus (Pigeon Arg r 1 No / CAG26895 Q5GQ85 833 tick) Artemia franciscana Art fr 5 Yes Myosin, light chain 1 ABS19977 A7L499 834 (Brine shrimp) Blattella germanica Bla g No / AAD13530 Q9UAM5 835 (German cockroach) 1.0101 Blattella germanica Bla g No / AAD13531 O96522 836 (German cockroach) 1.0201 Blattella germanica Bla g 2 No Aspartic protease AAA86744 P54958 837 (German cockroach) Blattella germanica Bla g 3 No Hemocyanin ACY40651 D0VNY7 838 (German cockroach) Blattella germanica Bla g 4 No Calycin AAA87851 P54962 839 (German cockroach) Blattella germanica Bla g 5 No Glutathione S-transferase AAB72147 O18598 840 (German cockroach) Blattella germanica Bla g No Troponin C, isoform 1 ABB89296 Q1A7B3 841 (German cockroach) 6.0101 Blattella germanica Bla g No Troponin C, isoform 2 ABB89297 Q1A7B2 842 (German cockroach) 6.0201 Blattella germanica Bla g No Troponin C, isoform 3 ABB89298 Q1A7B1 843 (German cockroach) 6.0301 Blattella germanica Bla g 7 No Tropomyosin AAF72534 Q9NG56 844 (German cockroach) Blattella germanica Bla g 8 No Myosin, light chain ABD47458 A0ERA8 845 (German cockroach) Blattella germanica Bla g 9 No Arginine kinase ABC86902 / 846 (German cockroach) Blattella germanica Bla g 11 No Alpha-amylase ABC68516 Q2L7A6 847 (German cockroach) Blomia tropicalis Blo t No Cysteine protease, isoform AK58415 Q95PJ4 848 (Storage mite) 1.0101 1 Blomia tropicalis Blo t No Cysteine protease, isoform AAQ24541 A1KXI0 849 (Storage mite) 1.0201 2 Blomia tropicalis Blo t No / AAQ73483 Q1M2P1 850 (Storage mite) 2.0101 Blomia tropicalis Blo t No / AAQ73482 Q1M2P2 851 (Storage mite) 2.0102 Blomia tropicalis Blo t No / AAQ73481 Q1M2P3 852 (Storage mite) 2.0103 Blomia tropicalis Blo t 3 No Trypsin AAM10779 Q8I916 853 (Storage mite) Blomia tropicalis Blo t 4 No Alpha amylase AAQ24543 A1KXI2 854 (Storage mite) Blomia tropicalis Blo t 5 No / AAD10850 O96870 855 (Storage mite) Blomia tropicalis Blo t 6 No Chymotrypsin AAQ24544 A1KXI3 856 (Storage mite) Blomia tropicalis Blo t 7 No Bactericidal permeability- ASX95438 / 857 (Storage mite) increasing like protein Blomia tropicalis Blo t 8 No Glutathione S-transferase ACV04860 C8CGT7 858 (Storage mite) Blomia tropicalis Blo t 10 No Tropomyosin ABU97466 A7XZI4 859 (Storage mite) Blomia tropicalis Blo t 11 No Paramyosin AAM83103 Q8MUF6 860 (Storage mite) Blomia tropicalis Blo t 12 No / AAA78904 Q17282 861 (Storage mite) Blomia tropicalis Blo t 13 No Fatty acid-binding protein AAC80579 Q17284 862 (Storage mite) Blomia tropicalis Blo t 19 No Anti-microbial peptide AHG97583 W5RZ24 863 (Storage mite) homologue Blomia tropicalis Blo t 21 No / AAX34047 A7IZE9 864 (Storage mite) Bombus Bom p 1 No Phospholipase A2 Q7M4I6 Q7M4I6 865 pennsylvanicus (Bumble bee) Bombus Bom p 4 No Protease Q7M4I3 Q7M4I3 866 pennsylvanicus (Bumble bee) Bombus terrestris Bom t 1 No Phospholipase A2 P82971 P82971 867 (Bumble bee) Bombus terrestris Bom t 4 No Protease P0CH88 P0CH88 868 (Bumble bee) Bombyx mori (Silk Bomb m Yes Arginine kinase ABB88514 Q2F5T5 869 moth) 1 Charybdis feriatus Cha f 1 Yes Tropomyosin AAF35431 Q9N2R3 870 (Crab) Chironomus kiiensis Chi k 10 No Tropomyosin CAA09938 O96764 871 (Midge) Chironomus thummi Chi t No Hemoglobin, component AAA28249 P02229 872 thummi (Midge) 1.0101 III Chironomus thummi Chi t No Hemoglobin, component AA25438 P02230 873 thummi (Midge) 1.0201 IV Chironomus thummi Chi t No Hemoglobin, component AAA80189 P02221 874 thummi (Midge) 2.0101 I/IA Chironomus thummi Chi t No Hemoglobin, component / P02221 874 thummi (Midge) 2.0201 I/IA (variant A113T) Chironomus thummi Chi t No Hemoglobin, components AAB58932 P02222 875 thummi (Midge) 3.0101 II-beta Chironomus thummi Chi t No Hemoglobin, components AAA69813 P02224 876 thummi (Midge) 3.0201 VI Chironomus thummi Chi t No Hemoglobin, components AAB58930 P02226 877 thummi (Midge) 3.0301 VIIA Chironomus thummi Chi t No Hemoglobin, components AAB58931 P02223 878 thummi (Midge) 3.0401 IX Chironomus thummi Chi t No Hemoglobin, components AAA28260 P12548 879 thummi (Midge) 3.0501 VIIB-3 Chironomus thummi Chi t No Hemoglobin, components AAA85491 P84296 880 thummi (Midge) 3.0601 VIIB-4 Chironomus thummi Chi t No Hemoglobin, components AAA69815 P84298 881 thummi (Midge) 3.0701 VIIB-9 Chironomus thummi Chi t No Hemoglobin, components AAA85486 P12549 882 thummi (Midge) 3.0702 VIIB-6 Chironomus thummi Chi t No Hemoglobin, components AAA85485 P12550 883 thummi (Midge) 3.0801 VIIB-7 Chironomus thummi Chi t No Hemoglobin, components P02227 P02227 884 thummi (Midge) 3.0901 VIII Chironomus thummi Chi t 4 No Hemoglobin, component P02231 P02231 885 thummi (Midge) IIIA Chironomus thummi Chi t 9 No Hemoglobin, component X P02228 P02228 886 thummi (Midge) Chortoglyphus arcuatus Cho a 10 No Tropomyosin AEX31649 / 887 (Storage mite) Crangon crangon Cra c 1 Yes Tropomyosin ACR43473 D7F1J4 888 (North Sea shrimp) Crangon crangon Cra c 2 Yes Arginine kinase ACR43474 D7F1J5 889 (North Sea shrimp) Crangon crangon Cra c 4 Yes Sarcoplasmic calcium- ACR43475 D7F1P9 890 (North Sea shrimp) binding protein Crangon crangon Cra c 5 Yes Myosin, light chain 1 ACR43477 D7F1Q1 891 (North Sea shrimp) Crangon crangon Cra c 6 Yes Troponin C ACR43478 D7F1Q2 892 (North Sea shrimp) Crangon crangon Cra c 8 Yes Triosephosphate isomerase ACR43476 D7F1Q0 893 (North Sea shrimp) Ctenocephalides felis Cte f 1 No Salivary antigen 1 AAC69105 Q94424 894 (Cat flea) Ctenocephalides felis Cte f 2 No Salivary allergen 2 AAF65314 Q9NH66 895 (Cat flea) Ctenocephalides felis Cte f 3 No Salivary allergen 3 / / / (Cat flea) Dermatophagoides Der f No Cysteine protease BAC53948 Q58A71 896 farinae (American 1.0101 (preproenzyme) house dust mite) Dermatophagoides Der f No Cysteine protease variant / Q3HWZ4 897 farinae (American 1.0102 (variant) house dust mite) Dermatophagoides Der f No Cysteine protease-1 BAC53948 P16311 898 farinae (American 1.0106 house dust mite) Dermatophagoides Der f No Cysteine protease ABL84749 A1YW11 899 farinae (American 1.0108 house dust mite) Dermatophagoides Der f No Cysteine protease ABL84750 A1YW12 900 farinae (American 1.0109 house dust mite) Dermatophagoides Der f No Vitellogenin ABL84751 A1YW13 901 farinae (American 1.0110 house dust mite) Dermatophagoides Der f No NPC2 family BAA01239 Q00855 902 farinae (American 2.0101 (variant) house dust mite) Dermatophagoides Der f No NPC2 family BAA01240 Q00855 903 farinae (American 2.0102 house dust mite) Dermatophagoides Der f No NPC2 family BAA01241 Q00855 903 farinae (American 2.0103 (variant) house dust mite) Dermatophagoides Der f No NPC2 family AAL47677 Q8WQK5 904 farinae (American 2.0105 house dust mite) Dermatophagoides Der f No NPC2 family CAI05848 Q5TIW2 905 farinae (American 2.0106 house dust mite) Dermatophagoides Der f No NPC2 family CAI05849 Q5TIW1 906 farinae (American 2.0107 house dust mite) Dermatophagoides Der f No NPC2 family CAI05850 Q5TIW0 907 farinae (American 2.0108 house dust mite) Dermatophagoides Der f No NPC2 family ABA39438 Q3HWZ2 908 farinae (American 2.0109 house dust mite) Dermatophagoides Der f No NPC2 family AAP35073 A1KXH0 909 farinae (American 2.0112 house dust mite) Dermatophagoides Der f No NPC2 family / A3F5F1 910 farinae (American 2.0116 house dust mite) Dermatophagoides Der f 3 No Trypsin BAA09920 P49275 911 farinae (American house dust mite) Dermatophagoides Der f 4 No alpha-amylase AHX03180 / 912 farinae (American house dust mite) Dermatophagoides Der f 6 No Chymotrypsin AAF28423 P49276 913 farinae (American house dust mite) Dermatophagoides Der f 7 No Bactericidal permeability- AAB35977 Q26456 914 farinae (American increasing like protein house dust mite) Dermatophagoides Der f 8 No Glutathione S-transferase AGC56215 / 915 farinae (American house dust mite) Dermatophagoides Der f 10 No Tropomyosin BAA04557 Q23939 916 farinae (American house dust mite) Dermatophagoides Der f 11 No Paramyosin AAK39511 Q967Z0 917 farinae (American house dust mite) Dermatophagoides Der f 13 No Fatty acid binding protein AAP35078 Q1M2P5 918 farinae (American house dust mite) Dermatophagoides Der f 14 No Apolipophorin BAA04558 Q94507 919 farinae (American house dust mite) Dermatophagoides Der f 15 No Chitinase AAD52672 Q9U6R7 920 farinae (American house dust mite) Dermatophagoides Der f 16 No Gelsolin/villin AAM64112 Q8MVU3 921 farinae (American house dust mite) Dermatophagoides Der f 17 No Calcium binding protein / / / farinae (American house dust mite) Dermatophagoides Der f 18 No Chitin-binding protein AAM19082 Q86R84 922 farinae (American house dust mite) Dermatophagoides Der f No / AIO08850.1 / 923 farinae (American 20.0101 house dust mite) Dermatophagoides Der f No Arginine kinase ABU97470.1 A7XZJ2 924 farinae (American 20.0201 house dust mite) Dermatophagoides Der f 21 No / AHC94806 B2GM84 925 farinae (American house dust mite) Dermatophagoides Der f 22 No / ABG35122 A5X5X4 926 farinae (American house dust mite) Dermatophagoides Der f 24 No Ubiquinol-cytochrome c AGI78542 M9RZ95 927 farinae (American reductase binding protein house dust mite) homologue Dermatophagoides Der f No Triosephosphate isomerase AGC56216 L7UZA7 928 farinae (American 25.0101 house dust mite) Dermatophagoides Der f No Triosephosphate isomerase AIO08860.1 / 929 farinae (American 25.0201 house dust mite) Dermatophagoides Der f 26 No Myosin alkali light chain AIO08852.1 / 930 farinae (American house dust mite) Dermatophagoides Der f 27 No Serpin AIO08851.1 / 931 farinae (American house dust mite) Dermatophagoides Der f No Heat Shock Protein AGC56218.1 L7V065 932 farinae (American 28.0101 house dust mite) Dermatophagoides Der f No Heat Shock Protein AIO08848.1 / 933 farinae (American 28.0201 house dust mite) Dermatophagoides Der f 29 No Peptidyl-prolyl cis-trans AAP35065 A1KXG2 934 farinae (American isomerase (cyclophilin) house dust mite) Dermatophagoides Der f 30 No Ferritin AGC56219.1 L7UZ91 935 farinae (American house dust mite) Dermatophagoides Der f 31 No Cofilin AIO08870.1 / 936 farinae (American house dust mite) Dermatophagoides Der f 32 No Secreted inorganic AIO08849.1 / 937 farinae (American pyrophosphatase house dust mite) Dermatophagoides Der f 33 No alpha-tubulin AIO08861 / 938 farinae (American house dust mite) Dermatophagoides Der f 34 No enamine/imine deaminase / / / farinae (American house dust mite) Dermatophagoides Der f 35 No / / / / farinae (American house dust mite) Dermatophagoides Der m 1 No Cysteine protease P16312 P16312 939 microceras (House dust mite) Dermatophagoides Der p No Cysteine protease AAB60215 P08176 940 pteronyssinus 1.0101 (variant) (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease AAB60215 P08176 941 pteronyssinus 1.0102 (European house dust mite) Dermatophagoides Der p No Cysteine protease AAB60215 P08176 940 pteronyssinus 1.0103 (variant) (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0104 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0105 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0106 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0107 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0108 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 940 pteronyssinus 1.0109 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 941 pteronyssinus 1.0110 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 940 pteronyssinus 1.0111 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / P08176 940 pteronyssinus 1.0112 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease ABA39435 Q3HWZ5 942 pteronyssinus 1.0113 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 942 pteronyssinus 1.0114 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0115 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 942 pteronyssinus 1.0116 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0117 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 942 pteronyssinus 1.0118 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0119 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0120 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0121 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0122 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease / Q3HWZ5 943 pteronyssinus 1.0123 (variant) (European house dust mite) Dermatophagoides Der p No Cysteine protease CAQ68250 C7T6L6 944 pteronyssinus 1.0124 (European house dust mite) Dermatophagoides Der p No NPC2 family AAF86462 P49278 945 pteronyssinus 2.0101 (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 946 pteronyssinus 2.0102 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 946 pteronyssinus 2.0103 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 945 pteronyssinus 2.0104 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 946 pteronyssinus 2.0105 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 945 pteronyssinus 2.0106 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 945 pteronyssinus 2.0107 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family / P49278 946 pteronyssinus 2.0108 (variant) (European house dust mite) Dermatophagoides Der p No NPC2 family CAQ68249 C7T6L5 947 pteronyssinus 2.0110 (European house dust mite) Dermatophagoides Der p No NPC2 family CAK22338 Q1H8P8 948 pteronyssinus 2.0114 (European house dust mite) Dermatophagoides Der p No NPC2 family CAQ68249 C7T6L5 947 pteronyssinus 2.0115 (European house dust mite) Dermatophagoides Der p 3 No Trypsin AAA19973 P39675 949 pteronyssinus (European house dust mite) Dermatophagoides Der p 4 No Alpha amylase AAD38942 Q9Y197 950 pteronyssinus (European house dust mite) Dermatophagoides Der p No / CAA35692 P14004 951 pteronyssinus 5.0101 (European house dust mite) Dermatophagoides Der p No / AAB32842 P14004 952 pteronyssinus 5.0102 (European house dust mite) Dermatophagoides Der p 6 No Chymotrypsin P49277 P49277 953 pteronyssinus (European house dust mite) Dermatophagoides Der p 7 No Bactericidal permeability- AAA80264 P49273 954 pteronyssinus increasing like protein (European house dust mite) Dermatophagoides Der p 8 No Glutathione S-transferase AAB32224 P46419 955 pteronyssinus (European house dust mite) Dermatophagoides Der p No Collagenolytic serine AAP57077 Q7Z163 956 pteronyssinus 9.0101 protease (European house dust mite) Dermatophagoides Der p No Collagenolytic serine AAN02511 Q8MWR4 957 pteronyssinus 9.0102 protease (European house dust mite) Dermatophagoides Der p 10 No Tropomyosin CAA75141 O18416 958 pteronyssinus (European house dust mite) Dermatophagoides Der p 11 No Paramyosin AAO73464 Q6Y2F9 959 pteronyssinus (European house dust mite) Dermatophagoides Der p 13 No Cytosolic Fatty Acid ADK92390 E0A8N8 960 pteronyssinus Binding Protein (European house dust mite) Dermatophagoides Der p 14 No Apolipophorin AAM21322 Q8N0N0 961 pteronyssinus (European house dust mite) Dermatophagoides Der p No Chitinase-like protein AAY84565 Q4JK69 962 pteronyssinus 15.0101 (European house dust mite) Dermatophagoides Der p No Chitinase-like protein AAY84564 Q4JK70 963 pteronyssinus 15.0201 (European house dust mite) Dermatophagoides Der p 18 No Chitin-binding protein AAY84563 Q4JK71 964 pteronyssinus (European house dust mite) Dermatophagoides Der p 20 No Arginine kinase ACD50950 B2ZSY4 965 pteronyssinus (European house dust mite) Dermatophagoides Der p 21 No / ABC73706 Q2L7C5 966 pteronyssinus (European house dust mite) Dermatophagoides Der p 23 No Peritrophin-like protein ACB46292 L7N6F8 967 pteronyssinus domain (PF01607) (European house dust mite) Dermatophagoides Der p 24 No biquinol-cytochrome c ALA65345.1 A0A0K2GUJ4 968 pteronyssinus reductase binding protein (European house dust mite) Dolichovespula Dol a 5 No Antigen 5 AAA28303 Q05108 969 arenaria (Yellow hornet) Dolichovespula Dol m No Phospholipase A1B CAA47341 Q06478 970 maculata (White face 1.0101 hornet) Dolichovespula Dol m No Phospholipase A1B P53357 P53357 971 maculata (White face 1.0102 hornet) Dolichovespula Dol m 2 No Hyaluronidase AAA68279 P49371 972 maculata (White face hornet) Dolichovespula Dol m No Venom Antigen 5 AA28301 P10736 973 maculata (White face 5.0101 hornet) Dolichovespula Dol m No Venom Antigen 5 AAA28302 P10737 974 maculata (White face 5.0102 hornet) Eriocheir sinensis Eri s 2 Yes ovary development-related AAO73305 Q5QKR2 975 (Eriocheir sinensis) protein Euroglyphus maynei Eur m No Cysteine protease AAC82351 P25780 976 (House dust mite) 1.0101 Euroglyphus maynei Eur m No Cysteine protease / P25780 976 (House dust mite) 1.0102 (variant) Euroglyphus maynei Eur m No NPC2 family AAC8234 Q9TZZ2 977 (House dust mite) 2.0101 Euroglyphus maynei Eur m No NPC2 family AC82350 Q9TZZ2 977 (House dust mite) 2.0102 (variant) Euroglyphus maynei Eur m 3 No Trypsin AAD10712 O97370 978 (House dust mite) Euroglyphus maynei Eur m 4 No Alpha-amylase AAD38943 Q9Y196 979 (House dust mite) Euroglyphus maynei Eur m 14 No Apolipophorin AAF14270 Q9U785 980 (House dust mite) Forcipomyia taiwana For t 1 No Serine/threonine-protein ACD65080 B2ZPG6 981 (Biting midge) kinase Forcipomyia taiwana For t 2 No Eukaryotic translation ACD65081 B2ZPG7 982 (Biting midge) initiation factor 3 subunit Glossina morsitans Glo m 5 No Tsetse antigen 5, CAP AAF82096 Q9NBA6 983 (Savannah Tsetse Fly) protein superfamily member Glycyphagus Gly d No Mite group 2 allergen CAB5997 Q9U5P7 984 domesticus (Storage 2.0101 mite) Glycyphagus Gly d No Mite group 2 allergen CAB76459 Q9NFQ4 985 domesticus (Storage 2.0201 mite) Harmonia axyridis Har a 1 No / / / / (Asian ladybeetle) Harmonia axyridis Har a 2 No aldehyde dehydrogenase / / / (Asian ladybeetle) Homarus americanus Hom a Yes Tropomyosin AAC48287 O44119-1 986 (American lobster) 1.0101 Homarus americanus Hom a Yes Tropomyosin AAC48288 O44119-2 987 (American lobster) 1.0102 Homarus americanus Hom a 3 Yes Myosin light chain 2 / / / (American lobster) Homarus americanus Hom a 6 Yes Troponin C P29291 P29291 988 (American lobster) Lepidoglyphus Lep d No / CAA61419 P80384 989 destructor (Storage 2.0101 mite) Lepidoglyphus Lep d No / CAD32313 P80384 990 destructor (Storage 2.0102 (variant) mite) Lepidoglyphus Lep d No / CAA58755 P80384 991 destructor (Storage 2.0201 (variant) mite) Lepidoglyphus Lep d No / CAD32314 P80384 992 destructor (Storage 2.0202 (variant) mite) Lepidoglyphus Lep d No / CAB62212 Q9U5P2 993 destructor (Storage 5.0101 mite) Lepidoglyphus Lep d No / AAQ73493 Q1M2N1 994 destructor (Storage 5.0102 mite) Lepidoglyphus Lep d No / AAQ73494 Q1M2N0 995 destructor (Storage 5.0103 mite) Lepidoglyphus Lep d 7 No Bactericidal permeability- CAB65963 Q9U1G2 996 destructor (Storage increasing like protein mite) Lepidoglyphus Lep d 10 No Tropomyosin CAB71342 Q9NFZ4 997 destructor (Storage mite) Lepidoglyphus Lep d 13 No Fatty acid-binding protein CAB62213 Q9U5P1 998 destructor (Storage mite) Lepisma saccharina Lep s 1 No Tropomyosin CAC84590 Q8T380 999 (Silverfish) Liposcelis Lip b 1 No unknown function P86712 P86712 1000 bostrychophila (Booklouse) Litopenaeus vannamei Lit v 1 Yes Tropomyosin ACB38288 B4YAH6 1001 (White shrimp) Litopenaeus vannamei Lit v 2 Yes Arginine kinase ABI98020 Q004B5 1002 (White shrimp) Litopenaeus vannamei Lit v 3 Yes Myosin, light chain 2 ACC76803 B7SNI3 1003 (White shrimp) Litopenaeus vannamei Lit v 4 Yes Sarcoplasmic calcium- ACM89179 C7A639 1004 (White shrimp) binding protein Macrobrachium Mac r 1 Yes tropomyosin ADC55380 D3XNR9 1005 rosenbergii (giant freshwater prawn) Melicertus latisulcatus Mel l 1 Yes tropomyosin AGF86397 M4M2H6 1006 (King Prawn) Metapenaeus ensis Met e 1 Yes tropomyosin AAA60330 Q25456 1007 (Shrimp) Myrmecia pilosula Myr p 1 No Pilosulin-1 CAA49760 Q07932 1008 (Australian jumper ant) Myrmecia pilosula Myr p 2 No pilosulin-3a AAB36316 Q26464 1009 (Australian jumper ant) Myrmecia pilosula Myr p 3 No pilosulin-4.1 BAD36780 Q68Y22 1010 (Australian jumper ant) Pachycondyla chinensis Pac c 3 No Antigen 5 ACA96507.1 C0ITL3 1011 (Asian needle ant) Pandalus borealis Pan b 1 Yes Tropomyosin CBY17558 E5BBS3 1012 (Northern shrimp) Panulirus stimpsoni Pan s 1 Yes Tropomyosin AAC38996 O61379 1013 (Spiny lobster) Penaeus aztecus Pen a 1 Yes Tropomyosin AAZ76743 Q3Y8M6 1014 (Brown shrimp) Penaeus indicus Pen i 1 Yes Tropomyosin / / / (Shrimp) Penaeus monodon Pen m 1 Yes tropomyosin ADM34184 A1KYZ2 1014 (Black tiger shrimp) Penaeus monodon Pen m 2 Yes arginine kinase AAO15713 Q8I9P7 1015 (Black tiger shrimp) Penaeus monodon Pen m 3 Yes Myosin light chain 2 ADM34185 E1A683 1016 (Black tiger shrimp) Penaeus monodon Pen m 4 Yes Sarcoplasmic calcium ADV17343 E7CGC4 1004 (Black tiger shrimp) binding protein Penaeus monodon Pen m 6 Yes Troponin C ADV17344 E7CGC5 1017 (Black tiger shrimp) Periplaneta americana Per a No Cr-PII allergen AAD13533 Q9TZR6 1018 (American cockroach) 1.0101 Periplaneta americana Per a No Cr-PII allergen AAC34312 O18535 1019 (American cockroach) 1.0102 Periplaneta americana Per a No Cr-PII allergen AAB82404 O18530 1020 (American cockroach) 1.0103 Periplaneta americana Per a No Cr-PII allergen AAC34737 O18528 1021 (American cockroach) 1.0104 Periplaneta americana Per a No Cr-PII allergen AAC34736 O18527 1022 (American cockroach) 1.0201 Periplaneta americana Per a 2 No aspartatic protease-like ADR82198 E7BQV5 1023 (American cockroach) Periplaneta americana Per a No Arylphorins/TO AAB09629 Q25641 1024 (American cockroach) 3.0101 Arthropod hemocyanins (Cr-PI Allergen) Periplaneta americana Per a No Arylphorins/TO AAB09632 Q94643 1025 (American cockroach) 3.0201 Arthropod hemocyanins (Cr-PI Allergen) Periplaneta americana Per a No Arylphorins/TO AAB62731 Q25640 1026 (American cockroach) 3.0202 Arthropod hemocyanins (Cr-PI Allergen) Periplaneta americana Per a No Arylphorins/TO AAB63595 Q25639 1027 (American cockroach) 3.0203 Arthropod hemocyanins (Cr-PI Allergen) Periplaneta americana Per a 6 No Troponin C AAX33730 Q1M0Y3 1028 (American cockroach) Periplaneta americana Per a 7 No Tropomyosin CAB38086 Q9UB83 1029 (American cockroach) Periplaneta americana Per a 9 No Arginine kinase ACA00204 / 1030 (American cockroach) Periplaneta americana Per a 10 No Serine protease AAX33734 Q1M0X9 1031 (American cockroach) Periplaneta americana Per a 11 No alpha amylase AKH04310 / 1032 (American cockroach) Periplaneta americana Per a 12 No Chitinase AKH04311 / 1033 (American cockroach) Plodia interpunctella Plo i 1 No Arginine kinase CAC85911 Q95PM9 1034 (Indianmeal moth) Plodia interpunctella Plo i 2 No Thioredoxin CBW45298 E1XUQ3 1035 (Indianmeal moth) Polistes annularis Pol a 1 No Phospholipase A1B AD52615 Q9U6W0 1036 (Wasp) Polistes annularis Pol a 2 No Hyaluronidase AAD52616 Q9U6V9 1037 (Wasp) Polistes annularis Pol a 5 No Antigen 5 AAA29793 Q05109 1038 (Wasp) Polistes dominulus Pol d No Phospholipase A1-1 AAS67041 Q6Q252 1039 (Mediterranean paper 1.0101 wasp) Polistes dominulus Pol d No Phospholipase A1-2 AAS67042 Q6Q251 1040 (Mediterranean paper 1.0102 wasp) Polistes dominulus Pol d No Phospholipase A1-3 AAS67043 Q6Q250 1041 (Mediterranean paper 1.0103 wasp) Polistes dominulus Pol d No Phospholipase A1-4 AAS67044 Q6Q249 1042 (Mediterranean paper 1.0104 wasp) Polistes dominulus Pol d 4 No Serine protease AAP37412 Q7Z269 1043 (Mediterranean paper wasp) Polistes dominulus Pol d 5 No Antigen 5 AAT95010 Q68KJ8 1044 (Mediterranean paper wasp) Polistes exclamans Pol e 1 No Phospholipase A1 / / / (Wasp) Polistes exclamans Pol e 4 No Serine protease / / / (Wasp) Polistes exclamans Pol e 5 No Antigen 5 AAT95009 Q68KJ9 1045 (Wasp) Polistes fuscatus Pol f 5 No Antigen 5 P35780 P35780 1046 (Wasp) Polistes gallicus (Wasp) Pol g 1 No Phospholipase A1 P83542 P83542 1047 Polistes gallicus (Wasp) Pol g 5 No Antigen 5 P83377 P83377 1048 Polistes metricus Pol m 5 No Antigen 5 P35780 P35780 1046 (Wasp) Polybia paulista (Wasp) Poly p 1 No Phospholipase A1 ABN13879 A2VBC4 1049 Polybia paulista (Wasp) Poly p 2 No Hyaluronidase / P86687 1050 Polybia paulista (Wasp) Poly p No Venom group 5 / C0HJV9 / 5.0101 Polybia paulista (Wasp) Poly p No Venom group 5 / P86686 1051 5.0102 Polybia scutellaris Poly s 5 No / / / (Wasp)

tastacus leptodactylus Pon l 4 Yes Sarcoplasmic calcium- P05946 P05946 1052 (Narrow-clawed binding protein crayfish)

tastacus leptodactylus Pon l 7 Yes Troponin I P05547 P05547 1053 (Narrow-clawed crayfish) Portunus pelagicus Por p 1 Yes Tropomyosin AGE44125 M1H607 1054 (Blue swimmer crab) Solenopsis geminata Sol g 2 No / / / / (Tropical fire ant) Solenopsis geminata Sol g 3 No / / / / (Tropical fire ant) Solenopsis geminata Sol g 4 No / AAF65312 Q9NH75 1055 (Tropical fire ant) Solenopsis invicta (Red Sol i 1 No Phospholipase A1B AAT95008 Q68KK0 1056 imported fire ant) Solenopsis invicta (Red Sol i 2 No / P35775 P35775 1057 imported fire ant) Solenopsis invicta (Red Sol i 3 No / AAB65434 P35778 1058 imported fire ant) Solenopsis invicta (Red Sol i 4 No / AAC97369 P35777 1059 imported fire ant) Solenopsis richteri Sol r 2 No / P35776 P35776 1060 (Black fire ant) Solenopsis richteri Sol r 3 No / P35779 P35779 1061 (Black fire ant) Solenopsis saevissima Sol s 2 No / ABC58726 A5X2H7 1062 (Brazilian fire ant) Solenopsis saevissima Sol s 3 No / / / / (Brazilian fire ant) Tabanus yao (Horsefly) Tab y 1 No Apyrase ADX78255 F1JZ10 1063 Tabanus yao (Horsefly) Tab y 2 No Hyaluronidase ADM18346 E0XKJ9 1064 Tabanus yao (Horsefly) Tab y 5 No Antigen 5-related protein, ADM18345 E0XKJ8 1065 CAP protein superfamily member Thaumetopoea Tha p 1 No / Q7M4K8 Q7M4K8 1066 pityocampa (Pine processionary moth) Thaumetopoea Tha p 2 No / P86360 P86360 1067 pityocampa (Pine processionary moth) Triatoma protracta Tria p 1 No Procalin AAF07903 Q9U6R6 1068 (California kissing bug) Tyrophagus Tyr p 2 No NPC2 family CAA73221 O02380 1069 putrescentiae (Storage mite) Tyrophagus Tyr p 3 No Trypsin ABZ81991 C6ZDB5 1070 putrescentiae (Storage mite) Tyrophagus Tyr p 10 No Tropomyosin AAT40866 Q6IUP9 1071 putrescentiae (Storage mite) Tyrophagus Tyr p 13 No Fatty-acid binding protein AAU11502 Q66RP5 1072 putrescentiae (Storage mite) Tyrophagus Tyr p 28 No Heat shock protein AOD75395.1 / 1073 putrescentiae (Storage mite) Tyrophagus Tyr p 34 No Troponin C ACL36923 D2DGW3 1074 putrescentiae (Storage mite) Tyrophagus Tyr p 35 No Aldehyde dehydrogenase AOD75396.1 / 1075 putrescentiae (Storage mite) Tyrophagus Tyr p 36 No Profilin AOD75399.1 / 1076 putrescentiae (Storage mite) Vespa crabro Vesp c 1 No Phospholipase A1B P0CH87 P0CH87 1077 (European hornet) Vespa crabro Vesp c No Antigen 5 P35781 P35781 1078 (European hornet) 5.0101 Vespa crabro Vesp c No Antigen 5 P35782 P35782 1079 (European hornet) 5.0102 Vespa magnifica Vesp ma No Hyaluronidase / / / (Hornet) 2 Vespa magnifica Vesp ma No Antigen 5, member of PR- / / / (Hornet) 5 1 family Vespa mandarinia Vesp m 1 No Phospholipase A1B / / / (Giant asian hornet) Vespa mandarinia Vesp m 5 No Antigen 5 P81657 P81657 1080 (Giant asian hornet) Vespula flavopilosa Ves f 5 No Antigen 5 P35783 P35783 1081 (Yellow jacket) Vespula germanica Ves g 5 No Antigen 5 CAJ28930 P35784 1082 (Yellow jacket) Vespula maculifrons Ves m 1 No Phospholipase A1B P51528 P51528 1083 (Yellow jacket) Vespula maculifrons Ves m 2 No Hyaluronidase P0CH89 P0CH89 1084 (Yellow jacket) Vespula maculifrons Ves m 5 No Antigen 5 P35760 P35760 1085 (Yellow jacket) Vespula pensylvanica Ves p 5 No Antigen 5 P35785 P35785 1086 (Yellow jacket) Vespula squamosa Ves s 1 No Phospholipase A1B P0CH86 P0CH86 1087 (Yellow jacket) Vespula squamosa Ves s 5 No Antigen 5 P35786 P35786 1088 (Yellow jacket) Vespula vidua (Wasp) Ves vi 5 No Antigen 5 P35787 P35787 1089 Vespula vulgaris Ves v 1 No Phospholipase A1B AAB48072 P49369 1090 (Yellow jacket) Vespula vulgaris Ves v No Hyaluronidase CAI77218 P49370 1091 (Yellow jacket) 2.0101 Vespula vulgaris Ves v No Hyaluronidase AAX14718 Q5D7H4 1092 (Yellow jacket) 2.0201 Vespula vulgaris Ves v 3 No Dipeptidylpeptidase IV ACA00159 B1A4F7 1093 (Yellow jacket) Vespula vulgaris Ves v 5 No Antigen 5 AAA30333 Q05110 1094 (Yellow jacket) Vespula vulgaris Ves v 6 No Vitellogenin AER70365 G8IIT0 1095 (Yellow jacket) Animalia Chordata Bos domesticus Bos Bos d No Lipocalin AAB08720 Q28133 1096 taurus (domestic cattle) 2.0101 Bos domesticus Bos Bos d No Lipocalin NP_777186 Q28133 1097 taurus (domestic cattle) 2.0102 Bos domesticus Bos Bos d 3 No S100 calcium-binding AAA91101 Q28050 1098 taurus (domestic cattle) protein A7 Bos domesticus Bos Bos d 4 Yes Alpha-lactalbumin AAA30615 P00711 1099 taurus (domestic cattle) Bos domesticus Bos Bos d 5 Yes Beta-lactoglobulin CAA32835 P02754 1100 taurus (domestic cattle) Bos domesticus Bos Bos d 6 Yes Serum albumin AAA51411 P02769 1101 taurus (domestic cattle) Bos domesticus Bos Bos d 7 Yes Immunoglobulin / / / taurus (domestic cattle) Bos domesticus Bos Bos d 8 Yes Caseins (see individual / / / taurus (domestic cattle) casein 9-12) Bos domesticus Bos Bos d 9 Yes alphaS1-casein NP_851372 P02662 1102 taurus (domestic cattle) Bos domesticus Bos Bos d 10 Yes alphaS2-casein NP_776953 P02663 1103 taurus (domestic cattle) Bos domesticus Bos Bos d 11 Yes beta-casein XP_005902099 P02666 1104 taurus (domestic cattle) Bos domesticus Bos Bos d 12 Yes kappa-casein NP_776719 P02668 1105 taurus (domestic cattle) Canis familiaris (dog) Can f 1 No Lipocalin AAC48794 O18873 1106 Canis familiaris (dog) Can f 2 No Lipocalin AAC48795 O18874 1107 Canis familiaris (dog) Can f 3 No Serum albumin BAC10663 P49822 1108 Canis familiaris (dog) Can f 4 No Lipocalin ACY38525 D7PBH4 1109 Canis familiaris (dog) Can f 5 No Arginine esterase, prostatic CAA68720 P09582 1110 kallikrein Canis familiaris (dog) Can f 6 No Lipocalin CCF72371 H2B3G5 1111 Canis familiaris (dog) Can f 7 No Epididymal Secretory AAB34263.1 Q28895 1112 Protein E1, or Niemann Pick type C2 protein Cavia porcellus (guinea Cav p 1 No Lipocalin P83507 P83507 1113 pig) Cavia porcellus (guinea Cav p 2 No Lipocalin CAX62129 F0UZ11 1114 pig) Cavia porcellus (guinea Cav p 3 No Lipocalin CAX62130 F0UZ12 1115 pig) Cavia porcellus (guinea Cav p 4 No Serum albumin AAQ20088 Q6WDN9 1116 pig) Cavia porcellus (guinea Cav p 6 No Lipocalin CAX62131 S0BDX9 1117 pig) Clupea harengus Clu h Yes Beta-parvalbumin CAQ72970 C6GKU6 1118 (Atlantic herring) 1.0101 Clupea harengus Clu h Yes Beta-parvalbumin CAQ72971 C6GKU7 1119 (Atlantic herring) 1.0201 Clupea harengus Clu h Yes Beta-parvalbumin CAQ72972 C6GKU8 1120 (Atlantic herring) 1.0301 Cyprinus carpio Cyp c Yes beta-parvalbumin CAC83658 Q8UUS3 1121 (Common carp) 1.0101 Cyprinus carpio Cyp c Yes beta-parvalbumin CAC83659 Q8UUS2 1122 (Common carp) 1.0201 Equus caballus Equ c 1 No Lipocalin AAC48691 Q95182 1123 (domestic horse) Equus caballus Equ c No Lipocalin P81216 P81216 1124 (domestic horse) 2.0101 Equus caballus Equ c No Lipocalin P81217 P81217 1125 (domestic horse) 2.0102 Equus caballus Equ c 3 No Serum albumin CAA52194 P35747 1126 (domestic horse) Equus caballus Equ c 4 No Latherin AAM09530 P82615 1127 (domestic horse) Felis domesticus (cat) Fel d 1 No Uteroglobin (chain 1) AAC37318 P30438 1128 (chain 1) (chain 1) Felis domesticus (cat) Fel d 1 No Uteroglobin (chain 2) AAC41616 P30440 1129 (chain 2) (chain 2) Felis domesticus (cat) Fel d 2 No Serum albumin CAA59279 P49064 1130 Felis domesticus (cat) Fel d 3 No Cystatin AAL49391 Q8WNR9 1131 Felis domesticus (cat) Fel d 4 No Lipocalin AAS77253 Q5VFH6 1132 Felis domesticus (cat) Fel d 5w No Immunoglobulin A / / / Felis domesticus (cat) Fel d 6w No Immunoglobulin M / / / Felis domesticus (cat) Fel d 7 No von Ebner gland protein ADK56160 E5D2Z5 1133 Felis domesticus (cat) Fel d 8 No Latherin-like protein ADM15668 F6K0R4 1134 Gadus callarias (Baltic Gad c 1 Yes Beta-parvalbumin P02622 P02622 1135 cod) Gadus morhua (Atlantic Gad m Yes Beta-parvalbumin AAK63086 Q90YL0 1136 cod) 1.0101 Gadus morhua (Atlantic Gad m Yes Beta-parvalbumin CAM56785 A5I873 1137 cod) 1.0102 Gadus morhua (Atlantic Gad m Yes Beta-parvalbumin AAK63087 Q90YK9 1138 cod) 1.0201 Gadus morhua (Atlantic Gad m Yes Beta-parvalbumin CAM56786 A5I874 1139 cod) 1.0202 Gadus morhua (Atlantic Gad m 2 Yes Beta-enolase B3A0L6 B3A0L6 1140 cod) Gadus morhua (Atlantic Gad m 3 Yes Fructose-bisphosphate P86980 P86980 1141 cod) aldolase A Gallus domesticus Gal d 1 Yes Ovomucoid P01005 P01005 1142 (chicken) Gallus domesticus Gal d 2 Yes Ovalbumin CAA23682 P01012 1143 (chicken) Gallus domesticus Gal d 3 Yes Ovotransferrin CAA26040 P02789 1144 (chicken) Gallus domesticus Gal d 4 Yes Lysozyme C CAA23711 P00698 1145 (chicken) Gallus domesticus Gal d 5 Yes Serum albumin CAA43098 P19121 1146 (chicken) Gallus domesticus Gal d 6 Yes YGP42 BAA13973 P87498 1147 (chicken) Gallus domesticus Gal d 7 Yes Myosin light chain 1f K02610.1 P02604 1148 (chicken) Gallus domesticus Gal d 8 Yes alpha-parvalbumin CAX32963 C1L370 1149 (chicken) Gallus domesticus Gal d 9 Yes Beta-enolase NP_990450 P07322 1150 (chicken) Gallus domesticus Gal d 10 Yes Aldolase / / / (chicken) Homo sapiens (human Hom s 1 No Squamous cell carcinoma BAA24056 O43290 1151 autoallergens) antigen SART-1 Homo sapiens (human Hom s 2 No Nascent polypeptide- AAK57544 Q13765 1152 autoallergens) associated complex alpha subunit Homo sapiens (human Hom s 3 No BCD7B protein CAA62012 Q13845 1153 autoallergens) Homo sapiens (human Hom s 4 No Atopy related autoantigen CAA76830 O75785 1154 autoallergens) CALC Homo sapiens (human Hom s 5 No Keratin, type II AAH69269 P02538 1155 autoallergens) cytoskeletal 6A Lates calcarifer Lat c Yes Beta 1-parvalbumin AHW83198 Q5IRB2 1156 (Barramundi) 1.0101 Lates calcarifer Lat c Yes Beta 2-parvalbumin AAT45383 Q6ITU9 1157 (Barramundi) 1.0201 Lepidorhombus Lep w 1 Yes Beta-parvalbumin CAP17694 B5WX08 1158 whiffiagonis (Megrim, Whiff, Turbot fish) Mesocricetus auratus Mes a 1 No lipocalin AAD55792 Q9QXU1 1159 (Golden hamster, Syrian hamster) Mus musculus (mouse) Mus m No Lipocalin/urinary CAA26953 P02762 1160 1.0101 prealbumin 6 Mus musculus (mouse) Mus m No Lipocalin/urinary AAA39768 P11589 1161 1.0102 prealbumin 2 Oncorhynchus keta Onc k 5 Yes beta-prime-component of BAJ07603 D5MU14 1162 (Chum salmon) vitellogenin Oncorhynchus mykiss Onc m Yes Beta1-parvalbumin P86431 P86431 1163 (Rainbow trout) 1.0101 Oncorhynchus mykiss Onc m Yes Beta2-parvalbumin P86432 P86432 1164 (Rainbow trout) 1.0201 Oreochromis Ore m 4 Yes Tropomyosin AFV53352 K4PEK4 1165 mossambicus (Mozambique tilapia) Oryctolagus cuniculus Ory c 1 No Lipocalin / / / (rabbit) Oryctolagus cuniculus Ory c No Lipophilin CL2 AAG42806 Q9GK63 1166 (rabbit) 3.A.0101 Oryctolagus cuniculus Ory c No Lipophilin AL AAG42802 Q9GK67 1167 (rabbit) 3.B.0101 Oryctolagus cuniculus Ory c 4 No Lipocalin CCC15303 U6C8D6 1168 (rabbit) Phodopus sungorus Phod s 1 No Lipocalin AGT28425 S5ZYD3 1169 (Siberian hamster) Rana esculenta (edible Ran e 1 Yes Alpha-parvalbumin CAC83046 Q8JIU2 1170 frog) Rana esculenta (edible Ran e 2 Yes Beta-parvalbumin CAC95152 Q8JIU1 1171 frog) Rastrelliger kanagurta Ras k 1 Yes Parvalbumin ANW10058 / 1172 (Indian Mackerel) Rattus norvegicus (Rat) Rat n 1 No Alpha-2u-globulin/ AAA41198 P02761 1173 Lipocalin Salmo salar (Atlantic Sal s 1 Yes Beta1-parvalbumin CAA66403 Q91482 1174 salmon) Salmo salar (Atlantic Sal s 2 Yes Beta-Enolase ACH70932 B5DGQ7 1175 salmon) Salmo salar (Atlantic Sal s 3 Yes Aldolase A ACH70901 B5DGM7 1176 salmon) Sardinops sagax Sar sa 1 Yes Beta-parvalbumin CAQ68366 B3WFF7 1177 (Pacific pilchard) Sebastes marinus Seb m Yes Beta-parvalbumin CAQ72968 C6GKU4 1178 (Ocean perch, redfish, 1.0101 snapper) Sebastes marinus Seb m Yes Beta-parvalbumin CAQ72969 C6GKU5 1179 (Ocean perch, redfish, 1.0201 snapper) Sus scrofa (Domestic Sus s 1 Yes Serum albumin AAA30988.1 P08835 1180 pig) Thunnus albacares Thu a 1 Yes Beta-parvalbumin CAQ72967 C6GKU3 1181 (Yellowfin tuna) Thunnus albacares Thu a 2 Yes Beta-enolase P86978 P86978 1182 (Yellowfin tuna) Thunnus albacares Thu a 3 Yes Aldolase A P86979 P86979 1183 (Yellowfin tuna) Xiphias gladius Xip g 1 Yes Beta-parvalbumin CAR48256 B9W4C2 1184 (Swordfish) Animalia Cnidaria and Mollusca Dendronephthya sp. Den n 1 No / / / / (Soft Coral) Crassostrea Cra g Yes tropomyosin ARX70262.1 / 1185 gigas (Pacific Ovster) 1.0101 Crassostrea Cra g Yes tropomyosin BAH10152.1 / 1186 gigas (Pacific Oyster) 1.0102 Haliotis laevigata × Hal l 1 Yes Tropomyosin APG42675 / 1187 Haliotis rubra (Jade tiger abaolone) Haliotis midae Hal m 1 Yes / / / / (Abalone) Helix aspersa (Brown Hel as 1 Yes Tropomyosin CAB3804 O97192 1188 garden snail) odes pacificus Tod p 1 Yes Tropomyosin / / / (Japanese flying squid) Animalia Nematoda Anisakis simplex Ani s 1 Yes unknown function, similar BAC77154 Q7Z1K3 1189 (Herring worm) to Kunitz serine protease inhibitors Anisakis simplex Ani s 2 Yes Paramyosin AAF72796 Q9NJA9 1190 (Herring worm) Anisakis simplex Ani s 3 Yes Tropomyosin CAB93501 Q9NAS5 1191 (Herring worm) Anisakis simplex Ani s 4 Yes Cysteine protease inhibitor CAK50389 Q14QT4 1192 (Herring worm) Anisakis simplex Ani s 5 Yes SXP/RAL-2 family protein BAF43534 A1IKL2 1193 (Herring worm) Anisakis simplex Ani s 6 Yes Serine protease inhibitor BAF43535 A1IKL3 1194 (Herring worm) Anisakis simplex Ani s 7 Yes UA3-recognized allergen ABL77410 A9XBJ8 1195 (Herring worm) Anisakis simplex Ani s 8 Yes SXP/RAL-2 family BAF75681 A7M6Q6 1196 (Herring worm) protein, isoform 1 Anisakis simplex Ani s 9 Yes SXP/RAL-2 family protein ABV55106 B2XCP1 1197 (Herring worm) Anisakis simplex Ani s 10 Yes Protein with unknown ACZ95445 D2K835 1198 (Herring worm) function Anisakis simplex Ani s 11 Yes Protein with unknown BAJ78220 E9RFF3 1199 (Herring worm) function Anisakis simplex Ani s 12 Yes Protein with unknown BAJ78223 E9RFF6 1200 (Herring worm) function Anisakis simplex Ani s 13 Yes Hemoglobin AFY98826 K9USK2 1201 (Herring worm) Anisakis simplex Ani s 14 Yes 3rd stage larval protein BAT62430 A0A0S3Q267 1202 (Herring worm) unknown function Ascaris lumbricoides Asc l 3 No Tropomyosin ACN32322 C0L3K2 1203 (Common roundworm) Ascaris lumbricoides Asc l 13 No lutathione S-transferase P46436 P46436 1204 (Common roundworm) (GST) Ascaris suum (Pig Asc s 1 No Polyprotein ABA-1 AAC06015 Q06811 1205 roundworm) Ascaris suum (Pig Asc s 13 No Glutathione transferase P46436 P46436 1204 roundworm) Fungi Ascomycota Alternaria alternata Alt a No / (major allergen) AAB47552 P79085 1206 (Alternaria plant rot 1.0101 fungus) Alternaria alternata Alt a No / (major allergen) AAS75297 Q6Q128 1207 (Alternaria plant rot 1.0102 fungus) Alternaria alternata Alt a 3 No Heat shock protein 70 AB48043 P78983 1208 (Alternaria plant rot fungus) Alternaria alternata Alt a 4 No Disulfide isomerase CAA58999 Q00002 1209 (Alternaria plant rot fungus) Alternaria alternata Alt a 5 No Ribosomal protein P2 AAB48041 P42037 1210 (Alternaria plant rot fungus) Alternaria alternata Alt a 6 No Enolase AAG42022 Q9HDT3 1211 (Alternaria plant rot fungus) Alternaria alternata Alt a 7 No YCP4 protein CAA55069 P42058 1212 (Alternaria plant rot fungus) Alternaria alternata Alt a 8 No Mannitol dehydrogenase AAO91800 P0C0Y4 1213 (Alternaria plant rot fungus) Alternaria alternata Alt a 10 No Aldehyde dehydrogenase CAA55071 P42041 1214 (Alternaria plant rot fungus) Alternaria alternata Alt a 12 No Acid ribosomal protein P1 CAA58998 P49148 1215 (Alternaria plant rot fungus) Alternaria alternata Alt a 13 No Glutathione-S-transferase AAR98813 Q6R4B4 1216 (Alternaria plant rot fungus) Alternaria alternata Alt a 14 No Manganese superoxide AGS80276 P86254 1217 (Alternaria plant rot dismutase fungus) Alternaria alternata Alt a 15 No Serine protease AHZ97469 A0A0F6N3V8 1218 (Alternaria plant rot fungus) Aspergillus flavus Asp fl 13 No Alkaline serine protease / / / (Cereal mold) Aspergillus fumigatus Asp f 1 No Mitogillin family AAB07779 P67875 1219 (Common mold) Aspergillus fumigatus Asp f 2 No / AAC69357 P79017 1220 (Common mold) Aspergillus fumigatus Asp f 3 No Peroxysomal protein AAB95638 O43099 1221 (Common mold) Aspergillus fumigatus Asp f 4 No / CAA04959 O60024 1222 (Common mold) Aspergillus fumigatus Asp f 5 No Extracellular CAA83015 P46075 1223 (Common mold) metalloproteinase Aspergillus fumigatus Asp f 6 No Mn superoxide dismutase AAB60779 Q92450 1224 (Common mold) Aspergillus fumigatus Asp f 7 No / CAA11255 O42799 1225 (Common mold) Aspergillus fumigatus Asp f 8 No Ribosomal protein P2 CAB64688 Q9UUZ6 1226 (Common mold) Aspergillus fumigatus Asp f 9 No / CAA11266 O42800 1227 (Common mold) Aspergillus fumigatus Asp f 10 No Aspartate protease CAA59419 Q12547 1228 (Common mold) Aspergillus fumigatus Asp f 11 No Peptidyl-prolyl isomerase CAB44442 Q9Y7F6 1229 (Common mold) Aspergillus fumigatus Asp f 12 No Heat shock protein P90 AAB51544 P40292 1230 (Common mold) Aspergillus fumigatus Asp f 13 No Alkaline serine protease CAA77666 P28296 1231 (Common mold) Aspergillus fumigatus Asp f 15 No / CAA05149 O60022 1232 (Common mold) Aspergillus fumigatus Asp f 16 No / CAAC61261 O74682 1233 (Common mold) Aspergillus fumigatus Asp f 17 No / CAA12162 O60025 1234 (Common mold) Aspergillus fumigatus Asp f 18 No Vacuolar serine protease CAA73782 P87184 1235 (Common mold) Aspergillus fumigatus Asp f 22 No Enolase AAK49451 Q96X30 1236 (Common mold) Aspergillus fumigatus Asp f 23 No L3 ribosomal protein AAM43909 Q8NKF4 1237 (Common mold) Aspergillus fumigatus Asp f 27 No Cyclophilin CAI78448 Q4WWX5 1238 (Common mold) Aspergillus fumigatus Asp f 28 No Thioredoxin CAI78449 Q1RQJ1 1239 (Common mold) Aspergillus fumigatus Asp f 29 No Thioredoxin CAI78450 Q4WV97 1240 (Common mold) Aspergillus fumigatus Asp f 34 No PhiA cell wall protein CAM54066 A4FSH5 1241 (Common mold) Aspergillus niger Asp n 14 No Beta-xylosidase AD13106 O93933 1242 (Black mold) Aspergillus niger Asp n 18 No Vacuolar serine protease / / / (Black mold) Aspergillus niger Asp n 25 No 3-phytase B AAA02934 P34754 1243 (Black mold) Aspergillus oryzae Asp o 13 No Alkaline serine protease CAA35594 P12547 1244 (Rice mold) Aspergillus oryzae Asp o 21 No TAKA-amylase A BAA00336 P10529 1245 (Rice mold) Aspergillus versicolor Asp v 13 No Extracellular alkaline ADE74975 D5LGB3 1246 serine protease Candida albicans Cand a 1 No Alcohol dehydrogenase CAA57342 P43067 1247 (Common yeast) Candida albicans Cand a 3 No Peroxysomal protein AAN11300 Q6YK78 1248 (Common yeast) Candida boidinii Cand b 2 No Peroxisomal membrane AAA34357 P14292 1249 (Yeast) protein A Cladosporium Cla c 9 No Vacuolar serine protease ABQ59329 B0L807 1250 cladosporioides Cladosporium Cla c 14 No Transaldolase ADK47394 G8Z407 1251 cladosporioides Cladosporium Cla h 2 No / / / / herbarum (Fungus of plants) Cladosporium Cla h 5 No Acid ribosomal protein P2 CAA55067 P42039 1252 herbarum (Fungus of plants) Cladosporium Cla h 6 No Enolase CAA55070 P42040 1253 herbarum (Fungus of plants) Cladosporium Cla h 7 No YCP4 protein CAA55068 P42059 1254 herbarum (Fungus of plants) Cladosporium Cla h 8 No Mannitol dehydrogenase AAO91801 P0C0Y5 1255 herbarum (Fungus of plants) Cladosporium Cla h 9 No Vacuolar serine protease AAX14379 B7ZK61 1256 herbarum (Fungus of plants) Cladosporium Cla h 10 No Aldehyde dehydrogenase CAA55072 P40108 1257 herbarum (Fungus of plants) Cladosporium Cla h 12 No Acid ribosomal protein P1 CAA59463 P50344 1258 herbarum (Fungus of plants) Curvularia lunata Cur l 1 No Serine protease / / / (Synonym: Cochliobolus lunatus) Curvularia lunata Cur l 2 No Enolase AAK67491 Q96VP4 1259 (Synonym: Cochliobolus lunatus) Curvularia lunata Cur l 3 No Cytochrome c AAK67492 Q96VP3 1260 (Synonym: Cochliobolus lunatus) Curvularia lunata Cur l 4 No Vacuolar serine protease ACF19589 B3V0K8 1261 (Synonym: Cochliobolus lunatus) Epicoccum Epi p 1 No Serine protease P83340 P83340 1262 purpurascens (Soil fungus) Fusarium culmorum Fus c 1 No Ribosomal protein P2 AAL79930 Q8TFM9 1263 (N.A.) Fusarium culmorum Fus c 2 No Thioredoxin-like protein AAL79931 Q8TFM8 1264 (N.A.) Fusarium proliferatum Fus p 4 No Transaldolase AHY02994 / 1265 Fusarium proliferatum Fus p 9 No Vacuolar serine protease AJA79001 A0A0U1Y1N5 1266 Penicillium Pen b 13 No Alkaline serine protease / / / brevicompactum (Penicillin) Penicillium Pen b 26 No Acidic ribosomal prot. P1 AAX11194 Q49KL9 1267 brevicompactum (Penicillin) Penicillium Pen ch No Alkaline serine protease AAF23726 Q9URR2 1268 chrysogenum 13 (Penicillin) Penicillium Pen ch No Vacuolar serine protease AAF71379 Q9P8G3 1269 chrysogenum 18 (Penicillin) Penicillium Pen ch No N-acetyl-glucosaminidase AAB34785 Q02352 1270 chrysogenum 20 (Penicillin) Penicillium Pen ch No Calreticulin AAX45072 Q2TL59 1271 chrysogenum 31 (Penicillin) Penicillium Pen ch No / ABP04053 B0L0W9 1272 chrysogenum 33 (Penicillin) Penicillium Pen ch No Transaldolase ADK27483 G8Z408 1273 chrysogenum 35 (Penicillin)

lium citrinum Pen c 3 No Peroxysomal membrane AAD42074 Q9Y8B8 1274 (Penicillin) protein

lium citrinum Pen c 13 No Alkaline serine protease Q9URH1 Q9URH1 1275 (Penicillin) (segment 1)

lium citrinum Pen c 19 No Heat shock protein P70 AAB06397 Q92260 1276 (Penicillin)

lium citrinum Pen c 22 No Enolase AAK51201 Q96X46 1277 (Penicillin)

lium citrinum Pen c 24 No elongation factor 1 beta AAR17475 Q69BZ7 1278 (Penicillin)

lium citrinum Pen c 30 No Catalase ABB89950 Q2V6Q5 1279 (Penicillin)

lium citrinum Pen c 32 No Pectate lyase ABM60783 A217W3 1280 (Penicillin) Penicillium crustosum Pen cr 26 No 60S acidic ribosomal AEX34122 H2E5X2 1281 phosphoprotein P1 Penicillium oxalicum Pen o 18 No vacuolar serine protease AAG44478 Q9HF12 1282 (Penicillin) Stachybotrys chartarum Sta c 3 No Extracellular alkaline Mg- ACT37324 C7E9W0 1283 dependent exodesoxyribonuclease Trichophyton rubrum Tri r 2 No Putative secreted alkaline AAD52013 Q9UW97 1284 protease Alp1 Trichophyton rubrum Tri r 4 No serine protease AAD52012 Q9UW98 1285 Trichophyton tonsurans Tri t 1 No / / / / Trichophyton tonsurans Tri t 4 No Serine protease P80514 P80514 1286 Fungi Basidiomycota and Zygomycota Coprinus comatus Cop c 1 No Leucine zipper protein CAB39376 Q9Y7G3 1287 (Shaggy mane) Coprinus comatus Cop c 2 No Thioredoxin CAB52130 Q9UW02 1288 (Shaggy mane) Coprinus comatus Cop c 3 No / CAB52131 Q9UW01 1289 (Shaggy mane) Coprinus comatus Cop c 5 No / CAB52132 Q9UW00 1290 (Shaggy mane) Coprinus comatus Cop c 7 No / CAB52133 Q9UVZ9 1291 (Shaggy mane) Malassezia furfur Mala f 2 No Peroxysomal membrane BAA32435 P56577 1292 (Pityriasis versicolor protein skin infection) Malassezia furfur Mala f 3 No Peroxysomal membrane BAA32436 P56578 1293 (Pityriasis versicolor protein skin infection) Malassezia furfur Mala f 4 No Mitochondrial malate AAD25927 Q9Y750 1294 (Pityriasis versicolor dehydrogenase skin infection) Malassezia sympodialis Mala s 1 No / CAA65341 Q01940 1295 (Skin fungus) Malassezia sympodialis Mala s 5 No / CAA09883 O93969 1296 (Skin fungus) Malassezia sympodialis Mala s 6 No Cyclophilin CAA09884 O93970 1297 (Skin fungus) Malassezia sympodialis Mala s 7 No / CAA09885 O93971 1298 (Skin fungus) Malassezia sympodialis Mala s 8 No / CAA09886 O93972 1299 (Skin fungus) Malassezia sympodialis Mala s 9 No / CAA09887 O93973 1300 (Skin fungus) Malassezia sympodialis Mala s No heat shock protein 70 CAD20981 Q8TGH3 1301 (Skin fungus) 10 Malassezia sympodialis Mala s No manganese superoxide CAD68071 Q873M4 1302 (Skin fungus) 11 dismutase Malassezia sympodialis Mala s No glucose-methanol-choline CAI43283 Q5GMY3 1303 (Skin fungus) 12 (GMC) oxidoreductase Malassezia sympodialis Mala s No Thioredoxin CAI78451 Q1RQI9 1304 (Skin fungus) 13 Psilocybe cubensis Psi c 1 No / / / / (Magic mushroom) Psilocybe cubensis Psi c 2 No Cyclophilin / / / (Magic mushroom) Rhodotorula Rho m 1 No Enolase AAP30720 Q870B9 1305 mucilaginosa (Yeast) Rhodotorula Rho m 2 No vacuolar serine protease AAT37679 Q32ZM1 1306 mucilaginosa (Yeast) Schizophyllum Sch c 1 No Glucoamylase XP_003030591 D8Q9M3 1307 commune Rhizopus oryzae (Bread Rhi o 1 No Aspartyl endopeptidase AIS82657 I1CLC6 1308 mold) Rhizopus oryzae (Bread Rhi o 2 No Cyclophilin ALM24136 / 1309 mold) Plantae Liliopsida Ananas comosus Ana c 1 Yes Profilin AAK54835 Q94JN2 1310 (Pineapple) Ananas comosus Ana c 2 Yes Bromelain BAA21849 O23791 1311 (Pineapple) Anthoxanthum Ant o 1 No Beta-expansin Q7M1X6 Q7M1X6 1312 odoratum (Sweet vernal grass) Asparagus officinalis Aspa o 1 Yes Non-specific lipid transfer / / / (Asparagus) protein type 1 Cocos nucifera Coc n 1 No vicilin-like protein ALQ56981.1 / 1313 (Coconut) Crocus sativus (Saffron Cro s 1 No / AAX93750 Q29W25 1314 crocus) Crocus sativus (Saffron Cro s 2 No Profilin AAW81034 Q5EF31 1315 crocus) Cynodon dactylon Cyn d No Beta-expansin AAB50734 O04701 1316 (Bermuda grass) 1.0101 Cynodon dactylon Cyn d No Beta-expansin AAK96255 Q947S7 1317 (Bermuda grass) 1.0201 Cynodon dactylon Cyn d No Beta-expansin AAL14077 Q947S6 1318 (Bermuda grass) 10202 Cynodon dactylon Cyn d No Beta-expansin AAL14079 Q947S4 1319 (Bermuda grass) 1.0203 Cynodon dactylon Cyn d No Beta-expansin AAF80379 Q9FVM0 1320 (Bermuda grass) 1.0204 Cynodon dactylon Cyn d 7 No Polcalcin CAA62634 P94092 1321 (Bermuda grass) Cynodon dactylon Cyn d 12 No Profilin CAA69670 O04725 1322 (Bermuda grass) Cynodon dactylon Cyn d 15 No pollen allergen(/) AAP80171 Q7XYF2 1323 (Bermuda grass) Cynodon dactylon Cyn d No enolase / / / (Bermuda grass) 22w Cynodon dactylon Cyn d 23 No / (pollen allergen) AAP80170 Q7XYF3 1324 (Bermuda grass) Cynodon dactylon Cyn d 24 No Pathogenesis-related AAU15051 Q647J6 1325 (Bermuda grass) protein PR-1 Dactylis glomerata Dac g 1 No Beta-expansin Q7M1X8 Q7M1X8 1326 (Orchard grass) Dactylis glomerata Dac g 2 No / AAB23303 Q41183 1327 (Orchard grass) Dactylis glomerata Dac g 3 No / AAB42200 P93124 1328 (Orchard grass) Dactylis glomerata Dac g 4 No / P82946 P82946 1329 (Orchard grass) Dactylis glomerata Dac g 5 No / / / / (Orchard grass) Festuca pratensis Fes p 4 No / / / / (Meadow fescue) Holcus lanatus (Velvet Hol l 1 No Beta-expansin CAA81610 P43216 1330 grass) Holcus lanatus (Velvet Hol l No Group V allergen CAB10765 O23972 1331 grass) 5.0101 Holcus lanatus (Velvet Hol l No Group V allergen CAB10766 O23971 1332 grass) 5.0201 Hordeum vulgare Hor v 5 No / AAB41585 O04828 1333 (Barley) Hordeum vulgare Hor v 12 No Profilin AAA92503 P52184 1334 (Barley) Hordeum vulgare Hor v 15 No Alpha-amylase inhibitor CAA45085 P16968 1335 (Barley) BMAI-1 precursor Hordeum vulgare Hor v 16 No Alpha-amylase / / / (Barley) Hordeum vulgare Hor v 17 No Beta-amylase / / / (Barley) Hordeum vulgare Hor v 20 No Gamma-hordein 3 CAA51204 P80198 1336 (Barley) Lolium perenne (Rye Lol p No Beta-expansin AAA63279 P14946 1337 grass) 1.0101 Lolium perenne (Rye Lol p No Beta-expansin CAB63699 Q9SC98 1338 grass) 1.0103 Lolium perenne (Rye Lol p 2 No / P14947 P14947 1339 grass) Lolium perenne (Rye Lol p 3 No / P14948 P14948 1340 grass) Lolium perenne (Rye Lol p 4 No / CAH92637 Q5TIW3 1341 grass) Lolium perenne (Rye Lol p 5 No / AAA33405 Q40237 1342 grass) Lolium perenne (Rye Lol p 11 No Ole e 1-related protein Q7M1X5 Q7M1X5 1343 grass) Musa acuminata Mus a 1 Yes Profilin AAK54834 Q94JN3 1344 (Banana) Musa acuminata Mus a 2 Yes Class 1 chitinase CAC81811 Q8VXF1 1345 (Banana) Musa acuminata Mus a 3 Yes Non-specific lipid transfer P86333 P86333 1346 (Banana) protein type 1 (nsLTP1) Musa acuminata Mus a 4 Yes Thaumatin-like protein 1Z3Q_A / 1347 (Banana) (Chain A) Musa acuminata Mus a 5 Yes Beta-1,3-glucanase / / / (Banana) Musa acuminata Mus a 6 Yes ascorbate peroxidase / / / (Banana) Oryza sativa (Rice) Ory s 1 No Beta-expansin AAA86533 Q40638 1348 Oryza sativa (Rice) Ory s 12 Yes Profilin A AAG32056 Q9FUD1 1349 Paspalum notatum Pas n 1 No Beta expansin ACA23876 B8PYF3 1350 (Bahia grass) Phalaris aquatica Pha a 1 No Beta-expansin AAB35984 Q41260 1351 (Canary grass) Phalaris aquatica Pha a 5 No / P56164 P56164 1352 (Canary grass) Phleum pratense Phl p No Beta-expansin CAA81613 Q40967 1353 (Timothy) 1.0101 Phleum pratense Phl p No Beta-expansin CAA55390 P43213 1354 (Timothy) 1.0102 Phleum pratense Phl p 2 No Grass group II/III CAA53529 P43214 1355 (Timothy) Phleum pratense Phl p No Berberine bridge enzyme CAD54670 Q5ZQK5 1356 (Timothy) 4.0101 Phleum pratense Phl p No Berberine bridge enzyme CAD54671 Q5ZQK4 1357 (Timothy) 4.0201 Phleum pratense Phl p No / CAA52753 Q40960 1358 (Timothy) 5.0101 Phleum pratense Phl p No / CAA50281 Q40962 1359 (Timothy) 5.0102 Phleum pratense Phl p No / AAC25994 O81341 1360 (Timothy) 5.0103 Phleum pratense Phl p No / CAB05372 P93467 1361 (Timothy) 5.0104 Phleum pratense Phl p No / AAC16525 O65318 1362 (Timothy) 5.0105 Phleum pratense Phl p No / AAC16526 O65319 1363 (Timothy) 5.0106 Phleum pratense Phl p No / AAC16528 O65321 1364 (Timothy) 5.0108 Phleum pratense Phl p No / CAD87529 Q84UI2 1365 (Timothy) 5.0109 Phleum pratense Phl p No / CAA81609 Q40963 1366 (Timothy) 5.0201 Phleum pratense Phl p No / CAB05371 P93466 1367 (Timothy) 5.0202 Phleum pratense Phl p No / AAC25995 O81342 1368 (Timothy) 5.0203 Phleum pratense Phl p No / AAC25997 O81343 1369 (Timothy) 5.0206 Phleum pratense Phl p No / AAC25998 O81344 1370 (Timothy) 5.0207 Phleum pratense Phl p No / CAA81608 P43215 1371 (Timothy) 6.0101 Phleum pratense Phl p No / CAA76556 O65868 1372 (Timothy) 6.0102 Phleum pratense Phl p 7 No Polcalcin CAA76887 O82040 1373 (Timothy) Phleum pratense Phl p 11 No Ole e 1-related protein AAN32987 Q8H6L7 1374 (Timothy) Phleum pratense Phl p No Profilin-1 CAA54686 P35079 1375 (Timothy) 12.0101 Phleum pratense Phl p No Profilin-2 CAA70608 O24650 1376 (Timothy) 12.0102 Phleum pratense Phl p No Profilin-3 CAA70609 O24282 1377 (Timothy) 12.0103 Phleum pratense Phl p 13 No Polygalacturonase CAB42886 Q9XG86 1378 (Timothy) Phoenix dactylifera Pho d 2 No Profilin CAD10390 Q8L5D8 1379 (Date palm) Poa pratensis Poa p 1 No Beta-expansin CAA10520 Q9ZP03 1380 (Kentucky blue grass) Poa pratensis Poa p 5 No / (pollen allergen) AAG42254 Q9FPR0 1381 (Kentucky blue grass) Secale cereale (Rye) Sec c 5 No Group 5 grass pollen CBG76811 F4MJM3 1382 allergen Secale cereale (Rye) Sec c Yes Gamma-70 SECALIN Q9S8B0 Q9S8B0 1383 20.0101 isoform S10-12 (COELIAC immunoreactive protein) Secale cereale (Rye) Sec c Yes Gamma-35 SECALIN Q9S8A7 Q9S8A7 1384 20.0201 isoform P13-14 (COELIAC immunoreactive protein) Secale cereale (Rye) Sec c 38 No Dimeric alpha- Q9S8H2 Q9S8H2 1385 amylase/trypsin inhibitor Sorghum halepense Sor h No Beta-expansin AIL01316 C5WMS3 1386 (Johnson grass) 1.0101 Sorghum halepense Sor h No Beta-expansin AIL01317 A0A077B4J2 1387 (Johnson grass) 1.0201 Sorghum halepense Sor h No Expansin-like protein; AIL01318 A0A077B7S9 1388 (Johnson grass) 2.0101 grass pollen group 2 allergen Sorghum halepense Sor h No Expansin-like protein; AIL01319 A0A077B2S0 1389 (Johnson grass) 2.0201 grass pollen group 2 allergen Sorghum halepense Sor h No Exopolygalacturonase AIL01320 A0A077B155 1390 (Johnson grass) 13.0101 (Glycosyl hydrolase 28) Sorghum halepense Sor h No Exopolygalacturonase AIL01321 A0A077B569 1391 (Johnson grass) 13.0201 (Glycosyl hydrolase 28) Triticum aestivum Tri a No Profilin-1 CAA61943 P49232 1392 (Wheat) 12.0101 Triticum aestivum Tri a No Profilin-2 CAA61944 P49233 1393 (Wheat) 12.0102 Triticum aestivum Tri a No Profilin-3 CAA61945 P49234 1394 (Wheat) 12.0103 Triticum aestivum Tri a No Profilin-4 CAQ57979 B6EF35 1395 (Wheat) 12.0104 Triticum aestivum Tri a 14 Yes Non-specific lipid transfer CAY54133 D2T2K2 1396 (Wheat) protein 1 Triticum aestivum Tri a 15 No Monomeric alpha-amylase CBA13560 D2TGC3 1397 (Wheat) inhibitor 0.28 Triticum aestivum Tri a 18 Yes Agglutinin isolectin 1 AAA34256 P10968 1398 (Wheat) Triticum aestivum Tri a 19 Yes Omega-5 gliadin, seed BAE20328 Q402I5 1399 (Wheat) storage protein Triticum aestivum Tri a 20 Yes Gamma gliadin BAN29066 Q9SYX8 1400 (Wheat) Triticum aestivum Tri a 21 No alpha-beta-gliadin CAY54134 D2T2K3 1401 (Wheat) Triticum aestivum Tri a 25 Yes Thioredoxin H CAB96931 Q9LDX4 1402 (Wheat) Triticum aestivum Tri a Yes High molecular weight CAA31395 P10388 1403 (Wheat) 26.0101 glutenin subunit Dx5 Triticum aestivum Tri a Yes High molecular weight AAZ23584 Q45R38 1404 (Wheat) 26.0201 glutenin subunit Bx7 Triticum aestivum Tri a 27 No Thiol reductase homologue BAC76688 Q7Y1Z2 1405 (Wheat) Triticum aestivum Tri a 28 No Dimeric alpha-amylase CAI84642 Q4W0V7 1406 (Wheat) inhibitor 0.19 Triticum aestivum Tri a No Tetrameric alpha-amylase CAZ76052 C7C4X0 1407 (Wheat) 29.0101 inhibitor CM1 Triticum aestivum Tri a No Tetrameric alpha-amylase CBA13559 D2TGC2 1408 (Wheat) 29.0201 inhibitor CM2 Triticum aestivum Tri a 30 No Tetrameric alpha-amylase CAA35597 P17314 1409 (Wheat) inhibitor CM3 Triticum aestivum Tri a 31 No Triosephosphate-isomerase CAC14917 Q9FS79 1410 (Wheat) Triticum aestivum Tri a 32 No 1-cys-peroxiredoxin AAQ74769 Q6W8Q2 1411 (Wheat) Triticum aestivum Tri a 33 No Serpin CAB52710 Q9ST57 1412 (Wheat) Triticum aestivum Tri a 34 No Glyceraldehyde-3- CAZ76054 C7C4X1 1413 (Wheat) phosphate-dehydrogenase Triticum aestivum Tri a 35 No Dehydrin CAY85463 D2TE72 1414 (Wheat) Triticum aestivum Tri a 36 Yes Low molecular weight AEH31546 B2Y2Q7 1415 (Wheat) glutenin GluB3-23 Triticum aestivum Tri a 37 Yes Alpha purothionin CAA65313 Q9T0P1 1416 (Wheat) Triticum aestivum Tri a 39 No Serine protease inhibitor- CCK33471 J7QW61 1417 (Wheat) like protein Triticum aestivum Tri a 40 No oform/methanol-soluble CAA42453.1 Q41540 1418 (Wheat) (CM) 17 protein [alpha amylase inhibitor] Triticum aestivum Tri a 41 Yes Mitochondrial ubiquitin AKJ77988.1 A0A0G3F2P1 1419 (Wheat) ligase activator of NFKB 1 Triticum aestivum Tri a 42 Yes Hypothetical protein from AKJ77986.1 A0A0G3F2F5 1420 (Wheat) cDNA Triticum aestivum Tri a 43 Yes Hypothetical protein from AKJ77987.1 A0A0G3F5F7 1421 (Wheat) cDNA Triticum aestivum Tri a 44 Yes Endosperm transfer cell AKJ77990.1 A0A0G3F720 1422 (Wheat) specific PR60 precursor Triticum aestivum Tri a 45 Yes Elongation factor 1 (EIF1) AKJ77985.1 A0A0G3F715 1423 (Wheat) Zea mays (Maize) Zea m 1 No Beta-expansin AAA33496 Q07154 1424 Zea mays (Maize) Zea m 8 Yes Chitinase ACX37090 P29022 1425 Zea mays (Maize) Zea m No Profilin-1 CAA51718 P35081 1426 12.0101 Zea mays (Maize) Zea m No Profilin-2 CAA51719 P35082 1427 12.0102 Zea mays (Maize) Zea m No Profilin-3 CAA51720 P35083 1428 12.0103 Zea mays (Maize) Zea m No Profilin-4 AAB86960 O22655 1429 12.0104 Zea mays (Maize) Zea m No Profilin-5 AAG35601 Q9FR39 1430 12.0105 Zea mays (Maize) Zea m Yes Non-specific lipid-transfer AAA33493 P19656-1 1431 14.0101 protein, isoform 1 Zea mays (Maize) Zea m Yes Non-specific lipid-transfer AAA33494 P19656-2 1432 14.0102 protein, isoform 2 Zea mays (Maize) Zea m 25 No thioredoxin CAI64400 Q4W1F7 1433 Plantae Magnoliopsida Acacia farnesiana Aca f 1 No Ole e 1-like protein AKV7266.1 A0A0K1SC24 1434 (Vachellia farnesiana) (Needle bush) Acacia farnesiana Aca f 2 No profilin AIV43662.1 A0A0A0RCW1 1435 (Vachellia farnesiana) (Needle bush) Actinidia chinensis Act c Yes Kiwellin P85261.1 P85261 1436 (Gold Kiwi fruit) 5.0101 Actinidia chinensis Act c Yes Kiwellin AGC39168.1 L7TT83 1437 (Gold Kiwi fruit) 5.0102 Actinidia chinensis Act c 8 Yes Pathogenesis-related CAM31908.1 D1YSM4 1438 (Gold Kiwi fruit) protein, PR-10, Bet v 1 family member Actinidia chinensis Act c 10 Yes Non-specific lipid-transfer P85204 P85204 1439 (Gold Kiwi fruit) protein 1 Actinidia deliciosa Act d 1 Yes Cysteine protease CAA34486 P00785 1440 (Green Kiwi fruit) (actinidin) Actinidia deliciosa Act d 2 Yes Thaumatin-like protein CAI38795 P81370 1441 (Green Kiwi fruit) Actinidia deliciosa Act d 3 Yes / P85063 P85063 1442 (Green Kiwi fruit) Actinidia deliciosa Act d 4 Yes Phytocystatin AAR92223 Q6TPK4 1443 (Green Kiwi fruit) Actinidia deliciosa Act d 5 Yes Kiwellin P84527 P84527 1444 (Green Kiwi fruit) Actinidia deliciosa Act d 6 Yes Pectin methylesterase BAC54964 P83326 1445 (Green Kiwi fruit) inhibitor Actinidia deliciosa Act d 7 Yes Pectin methylesterase P85076 P85076 1446 (Green Kiwi fruit) Actinidia deliciosa Act d 8 Yes Pathogenesis-related CAM31909 D1YSM5 1447 (Green Kiwi fruit) protein, PR-10, Bet v 1 family member Actinidia deliciosa Act d 9 Yes Profilin / / / (Green Kiwi fruit) Actinidia deliciosa Act d Yes Non-specific lipid-transfer P86137 P86137 1448 (Green Kiwi fruit) 10.0101 protein 1 Actinidia deliciosa Act d Yes Non-specific lipid-transfer P85206 P85206 1449 (Green Kiwi fruit) 10.0201 protein 2 Actinidia deliciosa Act d 11 Yes Major latex P85524 P85524 1450 (Green Kiwi fruit) protein/ripening-related protein (MLP/RRP), Bet v 1 family member Actinidia deliciosa Act d Yes Cupin, 11S globulin / C0HJF9.1 1451 (Green Kiwi fruit) 12.0101 Actinidia deliciosa Act d Yes Cupin, 11S globulin ABB77213 / 1452 (Green Kiwi fruit) 12.0102 Actinidia deliciosa Act d 13 Yes 2S albumin / / / (Green Kiwi fruit) Alnus glutinosa (Alder) Aln g 1 No Pathogenesis-related AAB24432 P38948 1453 protein, PR-10, Bet v 1 family member Alnus glutinosa (Alder) Aln g 4 No Polcalcin CAA76831 O81701 1454 Amaranthus retroflexus Ama r 1 No Ole e 1- like protein AKV72168 A0A0K1SC10 1455 (Redroot pigweed) Amaranthus retroflexus Ama r 2 No Profilin ACP43298 C3W2Q7 1456 (Redroot pigweed) Ambrosia artemisiifolia Amb a No Pectate lyase 5 AAA32665 P27759 1457 (Short ragweed) 1.0101 Ambrosia artemisiifolia Amb a No Pectate lyase 1 AAA32666 P27760 1458 (Short ragweed) 1.0201 Ambrosia artemisiifolia Amb a No Pectate lyase CBW30987 E1XUL3 1459 (Short ragweed) 1.0202 Ambrosia artemisiifolia Amb a No Pectate lyase 2 AAA32668 P27761 1460 (Short ragweed) 1.0301 Ambrosia artemisiifolia Amb a No Pectate lyase 2 / P27761 1460 (Short ragweed) 1.0302 (variant L48Y) Ambrosia artemisiifolia Amb a No Pectate lyase 2 AAA32669 P27761 1460 (Short ragweed) 1.0303 (variant H392R) Ambrosia artemisiifolia Amb a No Pectate lyase CBW30988 E1XUL4 1461 (Short ragweed) 1.0304 Ambrosia artemisiifolia Amb a No Pectate lyase CBW30989 E1XUL5 1462 (Short ragweed) 1.0305 Ambrosia artemisiifolia Amb a No Pectate lyase 3 AAA32670 P28744 1463 (Short ragweed) 1.0401 Ambrosia artemisiifolia Amb a No Pectate lyase CBW30993 E1XUL9 1464 (Short ragweed) 1.0402 Ambrosia artemisiifolia Amb a No Pectate lyase 4 AAA32671 P27762 1465 (Short ragweed) 1.0501 Ambrosia artemisiifolia Amb a No Pectate lyase CBW30995 E1XUM1 1466 (Short ragweed) 1.0502 Ambrosia artemisiifolia Amb a 3 No Plastocyanine P00304 P00304 1467 (Short ragweed) Ambrosia artemisiifolia Amb a 4 No Defensin-like protein CBK52317 D4IHC0 1468 (Short ragweed) Ambrosia artemisiifolia Amb a 5 No / P02878 P02878 1469 (Short ragweed) Ambrosia artemisiifolia Amb a 6 No Non-specific lipid transfer AAB51146 O04004 1470 (Short ragweed) protein type 1 Ambrosia artemisiifolia Amb a 7 No Plastocyanin / / / (Short ragweed) Ambrosia artemisiifolia Amb a No Profilin AAX77687 Q2KN24 1471 (Short ragweed) 8.0101 Ambrosia artemisiifolia Amb a No Profilin AAX77688 Q2KN23 1472 (Short ragweed) 8.0102 Ambrosia artemisiifolia Amb a No Polcalcin 9Calcium- AAX77684 Q2KN27 1473 (Short ragweed) 9.0101 binding protein isoallergen 1) Ambrosia artemisiifolia Amb a No Calcium-binding protein AAX77685 Q2KN26 1474 (Short ragweed) 9.0102 isoallergen 2 Ambrosia artemisiifolia Amb a No Polcalcin-like protein (4 AAX77686 Q2KN25 1475 (Short ragweed) 10 EF-hands) Ambrosia artemisiifolia Amb a No Cysteine protease AHA56102 V5LU01 1476 (Short ragweed) 11 Ambrosia artemisiifolia Amb a No Enolase ANZ22901.1 A0A1B2H9Q1 1477 (Short ragweed) 12.0101 Ambrosia artemisiifolia Amb a No Enolase ANZ22900 A0A1B2H9Q5 1478 (Short ragweed) 12.0102 Ambrosia psilostachya Amb p No / (pollen allergen) AAA20065 P43174 1479 (Western ragweed) 5.0101 Ambrosia psilostachya Amb p No / (pollen Allergen) AAA20064 P43175 1480 (Western ragweed) 5.0201 Ambrosia trifida (Giant Amb t 5 No / (pollen allergen) CAA39726 P10414 1481 ragweed) Anacardium Ana 0 Yes Vicilin-like protein AAM73730 Q8L5L5 1482 occidentale (Cashew) 1.0101 Anacardium Ana o Yes Vicilin-like protein AAM73729 Q8L5L6 1483 occidentale (Cashew) 1.0102 Anacardium Ana o 2 Yes Legumin-like protein AAN76862 Q8GZP6 1484 occidentale (Cashew) Anacardium Ana o 3 Yes 2s albumin AAL91665 Q8H2B8 1485 occidentale (Cashew) Apium graveolens Api g Yes Pathogenesis-related CAA88831 P49372 1486 (Celery) 1.0101 protein, PR-10, Bet v 1 family member, isoallergen 1 Apium graveolens Api g Yes Pathogenesis-related CAA99992 P92918 1487 (Celery) 1.0201 protein, PR-10, Bet v 1 family member, isoallergen 2 Apium graveolens Api g 2 Yes Non-specific lipid-transfer ACV04796 E6Y8S8 1488 (Celery) protein, type 1 Apium graveolens Api g 3 Yes Chlorophyll a-b binding CAA99993 P92919 1489 (Celery) protein, chloroplast Apium graveolens Api g 4 Yes Profilin AAD29409 Q9XF37 1490 (Celery) Apium graveolens Api g 5 Yes FAD-containing oxidase P81943 P81943 1491 (Celery) Apium graveolens Api g 6 Yes Non-specific lipid transfer P86809 P86809 1492 (Celery) protein type 2 Arachis hypogaea Ara h 1 Yes Cupin (Vicillin-type, 7S AAB00861 P43238 1493 (Peanut, groundnut) globulin) Arachis hypogaea Ara h 2 Yes Conglutin-7 (2S albumin), AAK96887 Q6PSU2 1494 (Peanut, groundnut) isoform 1 Arachis hypogaea Ara h Yes Cupin (Legumin-type, 11S AAC63045 O82580 1495 (Peanut, groundnut) 3.0101 globulin, Glycinin) Arachis hypogaea Ara h Yes Cupin (Legumin-type, 11S AAD47382 Q9SQH7 1496 (Peanut, groundnut) 3.0201 globulin, Glycinin) Arachis hypogaea Ara h 5 Yes Profilin AAD55587 Q9SQI9 1497 (Peanut, groundnut) Arachis hypogaea Ara h 6 Yes Conglutin (2S albumin) AAD56337 Q647G9 1498 (Peanut, groundnut) Arachis hypogaea Ara h Yes Conglutin (2S albumin) AAD56719 Q9SQH1 1499 (Peanut, groundnut) 7.0101 Arachis hypogaea Ara h Yes Conglutin (2S albumin) ABW17159 B4XID4 1500 (Peanut, groundnut) 7.0201 Arachis hypogaea Ara h Yes Pathogenesis-related AAQ91847 Q6VT83 1501 (Peanut, groundnut) 8.0101 protein, PR-10, Bet v 1 family member Arachis hypogaea Ara h Yes Pathogenesis-related ABP97433 B0YIU5 1502 (Peanut, groundnut) 8.0201 protein, PR-10, Bet v 1 family member Arachis hypogaea Ara h Yes Nonspecific lipid-transfer ABX56711 B6CEX8 1503 (Peanut, groundnut) 9.0101 protein type 1 Arachis hypogaea Ara h Yes Nonspecific lipid-transfer ABX75045 B6CG41 1504 (Peanut, groundnut) 9.0201 protein type 1 Arachis hypogaea Ara h Yes 16 kDa oleosin-1 AAU21499 Q647G5 1505 (Peanut, groundnut) 10.0101 Arachis hypogaea Ara h Yes 16 kDa oleosin-2 AAU21500 Q647G4 1506 (Peanut, groundnut) 10.0102 Arachis hypogaea Ara h Yes 14 kDa oleosin-1 AAZ20276 Q45W87 1507 (Peanut, groundnut) 11.0101 Arachis hypogaea Ara h Yes 14 kDa oleosin-2 AAZ20277 Q45W86 1508 (Peanut, groundnut) 11.0102 Arachis hypogaea Ara h 12 Yes Defensin / / / (Peanut, groundnut) Arachis hypogaea Ara h 13 Yes Defensin / / / (Peanut, groundnut) Arachis hypogaea Ara h Yes Oleosin, variant A AAK13449 Q9AXI1 1509 (Peanut, groundnut) 14.0101 Arachis hypogaea Ara h Yes Oleosin, variant B AAK13450 Q9AXI0 1510 (Peanut, groundnut) 14.0102 Arachis hypogaea Ara h Yes Oleosin AAT11925 Q6J1J8 1511 (Peanut, groundnut) 14.0103 Arachis hypogaea Ara h 15 Yes Oleosin AAU21501 Q647G3 1512 (Peanut, groundnut) Arachis hypogaea Ara h 16 Yes non-specific Lipid Transfer / / / (Peanut, groundnut) Protein 2 Arachis hypogaea Ara h 17 Yes non-specific Lipid Transfer / / / (Peanut, groundnut) Protein 1 Artemisia annua (Sweet Art an 7 No Galactose oxidase / / / Wormwood) Artemisia vulgaris Art v 1 No Defensin-like protein AAO24900 Q84ZX5 1513 (Mugwort, wormwood) Artemisia vulgaris Art v 2 No Pathogenesis-related CAK50834 A6GVD5 1514 (Mugwort, wormwood) protein PR-1 Artemisia vulgaris Art v No Nonspecific lipid transfer P0C088 P0C088 1515 (Mugwort, wormwood) 3.0101 protein type 1 Artemisia vulgaris Art v No Nonspecific lipid transfer ACE07186 C4MGG9 1516 (Mugwort, wormwood) 3.0201 protein type 1 Artemisia vulgaris Art v No Nonspecific lipid transfer ACE07187 C4MGH0 1517 (Mugwort, wormwood) 3.0202 protein type 1 Artemisia vulgaris Art v No Nonspecific lipid transfer ACE07188 C4MGH1 1518 (Mugwort, wormwood) 3.0301 protein type 1 Artemisia vulgaris Art v No Profilin-1 CAD12861 Q8H2C9 1519 (Mugwort, wormwood) 4.0101 Artemisia vulgaris Art v No Profilin-2 CAD12862 Q8H2C8 1520 (Mugwort, wormwood) 4.0201 Artemisia vulgaris Art v 5 No Polcalcin AAX85389 A0PJ17 1521 (Mugwort, wormwood) Artemisia vulgaris Art v 6 No Pectate lyase AAX85388 A0PJ16 1522 (Mugwort, wormwood) Bertholletia excelsa Ber e 1 Yes 2S sulfur-rich seed storage AAA33010 P04403 1523 (Brazil nut) albumin Bertholletia excelsa Ber e 2 Yes 11S globulin seed storage AAO38859 Q84ND2 1524 (Brazil nut) protein Beta vulgaris (Sugar Beta v 1 No Che a 1/Ole e 1 homolgue P85983 P85983 1525 beet) Beta vulgaris (Sugar Beta v 2 No Profilin, pollen P85984 P85984 1526 beet) Betula verrucosa Bet v No Pathogenesis-related CAA33887 P15494 1527 (Betula pendula) 1.0101 protein, PR-10, Bet v 1 (European white birch) family member 1-A Betula verrucosa Bet v No Pathogenesis-related CAA54482 P43177 1528 (Betula pendula) 1.0102 protein, PR-10, Bet v 1 (European white birch) family member 1-D/H Betula verrucosa Bet v No Pathogenesis-related CAA54483 P43178 1529 (Betula pendula) 1.0103 protein, PR-10, Bet v 1 (European white birch) family member 1-E Betula verrucosa Bet v No Pathogenesis-related CAA54484 P43179 1530 (Betula pendula) 1.0104 protein, PR-10, Bet v 1 (European white birch) family member 1-F/I Betula verrucosa Bet v No Pathogenesis-related CAA54485 P43180 1531 (Betula pendula) 1.0105 protein, PR-10, Bet v 1 (European white birch) family member 1-G Betula verrucosa Bet v No Pathogenesis-related CAA54487 P43183 1532 (Betula pendula) 1.0106 protein, PR-10, Bet v 1 (European white birch) family member 1-J Betula verrucosa Bet v No Pathogenesis-related CAA54489 P43185 1533 (Betula pendula) 1.0107 protein, PR-10, Bet v 1 (European white birch) family member 1-L Betula verrucosa Bet v No / (pollen allergen) CAB02155 Q96365 1534 (Betula pendula) 1.0108 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAB02156 Q96366 1535 (Betula pendula) 1.0109 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAB02157 Q96367 1536 (Betula pendula) 1.0110 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAB02158 Q96368 1537 (Betula pendula) 1.0111 (European white birch) Betula verrucosa Bet v No Pathogenesis-related CAB02159 P15494 1538 (Betula pendula) 1.0112 protein, PR-10, Bet v 1 (variant (European white birch) family member 1-A F63L) Betula verrucosa Bet v No / (pollen allergen) CAB02160 Q96370 1539 (Betula pendula) 1.0113 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAB02161 Q96371 1540 (Betula pendula) 1.0114 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAA96547 Q39431 1541 (Betula pendula) 1.0115 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAA04827.1 O23748 1542 (Betula pendula) 1.0116 (European white birch) Betula verrucosa Bet v No / (pollen allergen), isoform CAA07323.1 Q9SCI0 1543 (Betula pendula) 1.0117 at37 (European white birch) Betula verrucosa Bet v No / (pollen allergen), isoform CAA07329.1 Q9SCH6 1544 (Betula pendula) 1.0118 at5 (European white birch) Betula verrucosa Bet v No Major allergen Bet v 1.01E ABC41615.1 Q0QLS9 1545 (Betula pendula) 1.0119 (European white birch) Betula verrucosa Bet v No Pathogenesis-related CAA54421 P45431 1546 (Betula pendula) 1.0201 protein, PR-10, Bet v 1 (European white birch) family member 1-B Betula verrucosa Bet v No Pathogenesis-related CAA54481 P43176 1547 (Betula pendula) 1.0202 protein, PR-10, Bet v 1 (European white birch) family member 1-C Betula verrucosa Bet v No Pathogenesis-related CAA54488 P43184 1548 (Betula pendula) 1.0203 protein, PR-10, Bet v 1 (European white birch) family member 1-K Betula verrucosa Bet v No Pathogenesis-related CAA57550 P43186 1549 (Betula pendula) 1.0204 protein, PR-10, Bet v 1 (European white birch) family member 1-M/N Betula verrucosa Bet v No / (pollen allergen) CAA96540.1 Q39427 1550 (Betula pendula) 1.0205 (European white birch) Betula verrucosa Bet v No / (pollen allergen) CAA04828.1 O23749 1551 (Betula pendula) 1.0206 (European white birch) Betula verrucosa Bet v No Major allergen Bet v 1.02C ACF75030.1 Q0QLV2 1552 (Betula pendula) 1.0207 (European white birch) Betula verrucosa Bet v No 1 Sc-3 protein CAA54696.1 Q39415 1553 (Betula pendula) 1.0301 (European white birch) Betula verrucosa Bet v 2 No Profilin AAA16522 P25816 1554 (Betula pendula) (European white birch) Betula verrucosa Bet v 3 No Polcalcin-like protein (4 CAA55854 P43187 1555 (Betula pendula) EF-hand) (European white birch) Betula verrucosa Bet v 4 No Polcalcin CAA60628 Q39419 1556 (Betula pendula) (European white birch) Betula verrucosa Bet v No PhenylCoumaran benzylic AAC05116 O65002 1557 (Betula pendula) 6.0101 ether reductase (European white birch) Betula verrucosa Bet v No PhenylCoumaran benzylic AAG22740 Q9FUW6 1558 (Betula pendula) 6.0102 ether reductase (European white birch) Betula verrucosa Bet v 7 No Cyclophilin (Peptidyl- CAC84116 P81531 1559 (Betula pendula) prolyl cis-trans isomerase) (European white birch) Brassica juncea (Indian Bra j 1 Yes 2S albumin seed storage P80207 P80207 1560 or oriental mustard) protein Brassica napus Bra n 1 Yes 2S albumin seed storage P80208 P80208 1561 (Rapeseed) protein (Napin-3) Brassica oleracea Bra o 3 Yes non-specific lipid transfer / / / (Cabbage and others) protein type 1 Brassica rapa (Field Bra r 1 Yes 2S albumin CAA46782 Q42473 1562 mustard or Turnip) Brassica rapa (Field Bra r 2 Yes Prohevein homologue / P81729 1563 mustard or Turnip) (Chitin-binding allergen) Brassica rapa (Field Bra r 5 Yes Polcalcin BAA09634 P69197 1564 mustard or Turnip) Cannabis sativa (Indian Can s 3 No Non-specific lipid transfer CCK33472 W0U0V5 1565 hemp) protein type 1 Capsicum annuum Cap a 1 Yes Osmotin-like protein CAC34055 Q9ARG0 1566 (Chilli or bell pepper) (thaumatin-like protein) Capsicum annuum Cap a 2 Yes Profilin CAD10376 Q93YI9 1567 (Chilli or bell pepper) Carpinus betulus Car b No Pathogenesis-related CAA47366 P38949 1568 (Hornbeam) 1.0101 protein, PR-10, Bet v 1 family member 1A and 1B Carpinus betulus Car b No Pathogenesis-related CAA47357 P38949 1568 (Hornbeam) 1.0102 protein, PR-10, Bet v 1 (variant) family member 1A and 1B Carya illinoinensis Car i 1 Yes 2S albumin seed storage AAO32314 Q84XA9 1569 (Pecan) protein Carya illinoinensis Car i 2 Yes Vicilin-like protein ABV49590 B3STU4 1570 (Pecan) Carya illinoinensis Car i 4 Yes Legumin seed storage ABW86978 B5KVH4 1571 (Pecan) protein Castanea sativa Cas s 1 No Pathogenesis-related ACJ23861 B7TWE3 1572 (Chestnut) protein, PR-10, Bet v 1 family member Castanea sativa Cas s 5 Yes Chitinase AAB01895 Q42428 1573 (Chestnut) Castanea sativa Cas s 8 Yes Non-specific lipid transfer / / / (Chestnut) protein type 1 Castanea sativa Cas s 9 Yes Cytosolic class I small heat CAE46905 Q9ZS24 1574 (Chestnut) shock protein Catharanthus roseus Cat r 1 No Cyclophilin 9Peptidyl- CAA59468 I3QBM4 1575 (Rosy periwinkle) prolyl cis-trans isomerase) Chenopodium album Che a 1 No Ole e 1 homologue AAL07319 Q8LGR0 1576 (Lambsquarters) Chenopodium album Che a 2 No Profilin AAL92870 Q84V37 1577 (Lambsquarters) Chenopodium album Che a 3 No Polcalcin AAL92871 Q84V36 1578 (Lambsquarters) Citrullus lanatus Citr l 2 Yes Profilin AAU43733 Q5XWE1 1579 (watermellon) Citrus limon (Lemon) Cit l 3 Yes Non-specific lipid-transfer P84160 P84160 1580 protein Citrus reticulata Cit r 3 Yes Non-specific lipid transfer P84161 P84161 1581 (Tangerine) protein type 1 Citrus sinensis (Sweet Cit s 1 Yes Germin-like protein P84159 P84159 1582 orange) Citrus sinensis (Sweet Cit s 2 Yes Profilin CAI23765 P84177 1583 orange) Citrus sinensis (Sweet Cit s 3 Yes Non-specific lipid-transfer CAH03799 Q6EV47 1584 orange) protein type 1 Citrus sinensis (Sweet Cit s 7 Yes Gibberellin regulated / / / orange) protein Coffea arabica (Arabian Cof a 1 No Class III chitinase ADH10372 D7REL9 1585 coffee) Coffea arabica (Arabian Cof a 2 No Metallothionein type 2 AGL34967 AGL34967 1586 coffee) Coffea arabica (Arabian Cof a 3 No Metallothionein type 3 AGL34968 R4MUV4 1587 coffee) Corylus avellana Cor a Yes Pathogenesis-related CAA50327 Q08407 1588 (Hazelnut) 1.0101 protein, PR-10, Bet v 1 family member; isoform 5, 6, 11 and 16 Corylus avellana Cor a Yes Pathogenesis-related CAA96548 Q39453 1589 (Hazelnut) 1.0201 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Pathogenesis-related CAA96549 Q39454 1590 (Hazelnut) 1.0301 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Pathogenesis-related AAD48405 Q9SWR4 1591 (Hazelnut) 1.0401 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Pathogenesis-related AAG40329 Q9FPK4 1592 (Hazelnut) 1.0402 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Pathogenesis-related AAG40330 Q9FPK3 1593 (Hazelnut) 1.0403 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Pathogenesis-related AAG40331 Q9FPK2 1594 (Hazelnut) 1.0404 protein, PR-10, Bet v 1 family member Corylus avellana Cor a Yes Profilin AAK01235 Q9AXH5 1595 (Hazelnut) 2.0101 Corylus avellana Cor a Yes Profilin AAK01236 Q9AXH4 1596 (Hazelnut) 2.0102 Corylus avellana Cor a 6 No Isoflavone reductase / / / (Hazelnut) homologue Corylus avellana Cor a 8 Yes Non-specific lipid transfer AAK28533 Q9ATH2 1597 (Hazelnut) protein type 1 Corylus avellana Cor a 9 Yes 11S seed storage globulin AAL73404 Q8W1C2 1598 (Hazelnut) (legumin-like) Corylus avellana Cor a 10 No Luminal binding protein CAC14168 Q9FSY7 1599 (Hazelnut) Corylus avellana Cor a 11 Yes 7S seed storage globulin AAL86739 Q8S4P9 1600 (Hazelnut) (vicilin-like) Corylus avellana Cor a 12 Yes 17 kDa oelosin AAO67349 Q84T21 1601 (Hazelnut) Corylus avellana Cor a 13 Yes 14-16 kDa oleosin AAO65960 Q84T91 1602 (Hazelnut) Corylus avellana Cor a 14 Yes 2S albumin ACO56333 D0PWG2 1603 (Hazelnut) Cucumis melo Cuc m 1 Yes Alkaline serine protease BAA06905 Q39547 1604 (Muskmelon) (cucumisin) Cucumis melo Cuc m 2 Yes Profilin AAW69549 Q5FX67 1605 (Muskmelon) Cucumis melo Cuc m 3 Yes Pathogenesis-related P83834 P83834 1606 (Muskmelon) protein PR-1 Daucus carota (Carrot) Dau c Yes Pathogenesis-related AAB01092 O04298 1607 1.0101 protein, PR-10, Bet v 1 family member Daucus carota (Carrot) Dau c Yes Pathogenesis-related AAL76932 Q8SAE7 1608 1.0201 protein, PR-10, Bet v 1 family member Daucus carota (Carrot) Dau c Yes PRP-like protein ADL32660 D9ZHN9 1609 1.0301 Daucus carota (Carrot) Dau c 4 Yes Profilin AAL76933 Q8SAE6 1610 Daucus carota (Carrot) Dau c 5 Yes Isoflavone reductase-like AEY79728 H2DF86 1611 protein Fagopyrum esculentum Fag e 2 Yes 2S albumin ABC18306 Q2PS07 1612 (Common buckwheat) Fagopyrum esculentum Fag e 3 Yes Vicilin ABQ10638 A5HIX6 1613 (Common buckwheat) Fagopyrum esculentum Fag e Yes Antimicrobial Peptide / P0DKH7 1614 (Common buckwheat) 4.0101 Fagopyrum esculentum Fag e Yes Antimicrobial Peptide / P0DKH8 1615 (Common buckwheat) 4.0102 Fagopyrum esculentum Fag e 5 Yes Vicilin-like protein AY536051.1 Q6QJL1 1616 (Common buckwheat) Fagopyrum tataricum Fag t 2 Yes 2S albumin ADW27428 E9NX73 1617 (Tartarian buckwheat) Fagus sylvatica Fag s 1 No Pathogenesis-related ACJ23864 B7TWE6 1618 (European beech) protein, PR-10, Bet v 1 family member Fragaria ananassa Fra a 1 Yes Pathogenesis-related CAJ29538.1 Q3T923 1619 (Strawberry) protein, PR-10, Bet v 1 family member Fragaria ananassa Fra a Yes Non-specific lipid transfer CAC86258 Q8VX12 1620 (Strawberry) 3.0101 protein type 1 (ltp6) Fragaria ananassa Fra a Yes Non-specific lipid transfer AAY83342 Q4PLT9 1621 (Strawberry) 3.0102 protein type 1 (ltp2) Fragaria ananassa Fra a Yes Non-specific lipid transfer AAY83341 Q4PLU0 1622 (Strawberry) 3.0201 protein type 1 (ltp1) Fragaria ananassa Fra a Yes Non-specific lipid transfer AAY83345 Q4PLT6 1623 (Strawberry) 3.0202 protein type 1 (ltp5) Fragaria ananassa Fra a 4 Yes Profolin XP_004287490 P0C0Y3 1624 (Strawberry) Fraxinus excelsior Fra e No Ole e 1-like protein family AAQ08947 Q7XAV4 1625 (Ash) 1.0101 member Fraxinus excelsior Fra e No Ole e 1-like protein family AAV74343 Q5EXJ6 1626 (Ash) 1.0102 member Fraxinus excelsior Fra e No Ole e 1-like protein family AAQ83588 Q6U740 1627 (Ash) 1.0201 member Glycine max (Soybean) Gly m 1 No Hydrophobic protein from Q9S8F3 Q9S8F3 1628 soybean Glycine max (Soybean) Gly m 2 No Defensin / / / Glycine max (Soybean) Gly m Yes Profilin-1 CAA11756 O65809 1629 3.0101 Glycine max (Soybean) Gly m Yes Profilin-2 CAA11755 O65810 1630 3.0102 Glycine max (Soybean) Gly m 4 Yes Stress-induced protein CAA42646 P26987 1631 SAM22 Glycine max (Soybean) Gly m Yes alpha subunit of Beta- BAA23360 O22120 1632 5.0101 conglycinin (vicilin, 7S globulin) Glycine max (Soybean) Gly m Yes alpha subunit of Beta- BAA74452 Q9FZP9 1633 5.0201 conglycinin (vicilin, 7S globulin) Glycine max (Soybean) Gly m Yes beta chain of Beta- AAB23463 P25974 1634 5.0301 conglycinin (variant F36L V51G F197L) Glycine max (Soybean) Gly m Yes Glycinin G1 (legumin, 11S BAC78522 P04776 1635 6.0101 globulin) Glycine max (Soybean) Gly m Yes Glycinin G2 BAA00154 P04405 1636 6.0201 Glycine max (Soybean) Gly m Yes Glycinin G3 CAA33217 P11828 1637 6.0301 Glycine max (Soybean) Gly m Yes Glycinin BAA74953 Q9SB11 1638 6.0401 Glycine max (Soybean) Gly m Yes Glycinin A3B4 subunit BAB15802 Q7GC77 1639 6.0501 Glycine max (Soybean) Gly m 7 Yes Seed biotinylated protein ACS49840 C6K8D1 1640 Glycine max (Soybean) Gly m 8 Yes 2S albumin AAB71140 P19594 1641 Helianthus annuus Hel a 1 No / / / / (Sunflower) Helianthus annuus Hel a 2 No Profilin CAA75506 O81982 1642 (Sunflower) Helianthus annuus Hel a 3 Yes Non-specific lipid transfer AAP47226 Q7X9Q5 1643 (Sunflower) protein type 1 Hevea brasiliensis (Para Hev b 1 No Rubber elongation factor CAA39880 P15252 1644 rubber tree (latex)) Hevea brasiliensis (Para Hev b 2 No beta-1,3-glucanase, basic AAA87456 P52407 1645 rubber tree (latex)) vacuolar isoform Hevea brasiliensis (Para Hev b 3 No Small rubber particle AAC82355 O82803 1646 rubber tree (latex)) protein Hevea brasiliensis (Para Hev b 4 No Lecithinase homologue AAR98518 Q6T4P0 1647 rubber tree (latex)) Hevea brasiliensis (Para Hev b 5 No / AAC49447 Q39967 1648 rubber tree (latex)) Hevea brasiliensis (Para Hev b 6 No Hevein precursor AAA33357 P02877 1649 rubber tree (latex)) Hevea brasiliensis (Para Hev b 7 No Patatin-like protein AAC27724 O04008 1650 rubber tree (latex)) Hevea brasiliensis (Para Hev b No Profilin-1 CAA75312 O65812 1651 rubber tree (latex)) 8.0101 Hevea brasiliensis (Para Hev b No Profilin-2 CAB51914 Q9STB6 1652 rubber tree (latex)) 8.0102 Hevea brasiliensis (Para Hev b No Profilin-3 AAF34341 Q9M7N0 1653 rubber tree (latex)) 8.0201 Hevea brasiliensis (Para Hev b No Profilin-4 AAF34342 Q9M7M9 1654 rubber tree (latex)) 8.0202 Hevea brasiliensis (Para Hev b No Profilin-5 AAF34343 Q9M7M8 1655 rubber tree (latex)) 8.0203 Hevea brasiliensis (Para Hev b No Profilin-6 CAB96215 Q9LEI8 1656 rubber tree (latex)) 8.0204 Hevea brasiliensis (Para Hev b 9 No Enolase CAC00532 Q9LEJ0 1657 rubber tree (latex)) Hevea brasiliensis (Para Hev b No Superoxide dismutase AAA16792 P35017 1658 rubber tree (latex)) 10.0101 (Mn), mitochondrial Hevea brasiliensis (Para Hev b No Superoxide dismutase CAB53458 Q9STB5 1659 rubber tree (latex)) 10.0102 Hevea brasiliensis (Para Hev b No Superoxide dismutase CAC13961 Q9FSJ2 1660 rubber tree (latex)) 10.0103 Hevea brasiliensis (Para Hev b No Class I chitinase CAC42881 Q949H3 1661 rubber tree (latex)) 11.0101 Hevea brasiliensis (Para Hev b No Class I chitinase CAD24068 Q8GUD7 1662 rubber tree (latex)) 11.0102 Hevea brasiliensis (Para Hev b 12 No Non-specific lipid transfer AAL25839 Q8RYA8 1663 rubber tree (latex)) protein type 1 Hevea brasiliensis (Para Hev b 13 No Esterase AAP37470 Q7Y1X1 1664 rubber tree (latex)) Hevea brasiliensis (Para Hev b 14 No Hevamine ADR82196 E7BQV3 1665 rubber tree (latex)) Hevea brasiliensis (Para Hev b 15 No Serine protease inhibitor CCW27997 W0USW9 1666 rubber tree (latex)) Humulus japonicus Hum j 1 No / AAP94213 Q7XBE3 1667 (Japanese hop) Juglans nigra (Black Jug n 1 Yes 2S albumin seed storage AAM54365 Q7Y1C2 1668 walnut) protein Juglans nigra (Black Jug n 2 Yes Vicilin seed storage protein AAM54366 Q7Y1C1 1669 walnut) Juglans nigra (Black Jug n 4 Yes Legumin / / / walnut) Juglans regia (English Jug r 1 Yes 2S albumin seed storage AAB41308 P93198 1670 walnut) protein Juglans regia (English Jug r 2 Yes Vicilin seed storage protein AAF18269 Q9SEW4 1671 walnut) Juglans regia (English Jug r 3 Yes Non-specific lipid transfer ACI47547 C5H617 1672 walnut) protein type 1 Juglans regia (English Jug r 4 Yes 11S globulin seed storage AAW29810 Q2TPW5 1673 walnut) protein Juglans regia (English Jug r 5 Yes Pathogenesis Related APD76154.1 / 1674 walnut) protein-10 Juglans regia (English Jug r 6 Yes vicilin-like cupin / / / walnut) Kochia scoparia Koc s 1 No Ole e 1-like protein AKV72169 A0A0K1SC44 1675 (Burning bush) Kochia scoparia Koc s 2 No profilin AIV43661.1 / 1676 (Burning bush) Lactuca sativa Lac s 1 Yes Non-specific lipid transfer / / / (Cultivated lettuce) protein Lens culinaris (Lentil) Len c Yes Gamma-vicilin subunit CAD87730 Q84UI1 1677 1.0101 Lens culinaris (Lentil) Len c Yes Gamma-vicilin subunit CAD87731 Q84UI0 1678 1.0102 Lens culinaris (Lentil) Len c 2 Yes Seed-specific biotinylated / / / protein Lens culinaris (Lentil) Len c 3 Yes Nonspecific lipid transfer AAX35807 A0AT29 1679 protein type 1 Ligustrum vulgare Lig v 1 No Ole e 1-like protein family CAA54818 O82015 1680 (Common privet) member Litchi chinensis Lit c 1 Yes Profilin AAL07320 Q941H7 1681 (Lychee) Lupinus (albus ) Lup a 5 Yes Profilin / / / Lupinus angustifolius Lup an 1 Yes Conglutin beta (7S seed ACB05815 B8Q5G0 1682 (Narrow-leaved blue storage globulin, vicilin) lupin) Malus domestica Mal d Yes Pathogenesis-related CAA58646 P43211 1683 (Apple) 1.0101 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26546 Q9SYV2 1684 (Apple) 1.0103 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26552 Q9SYV5 1685 (Apple) 1.0104 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26553 Q9SYV6 1686 (Apple) 1.0105 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26554 Q9SYV7 1687 (Apple) 1.0106 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26555 Q9SYV8 1688 (Apple) 1.0107 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD29671 Q9SYW3 1689 (Apple) 1.0108 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAK13029 Q941P6 1690 (Apple) 1.0109 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAB01362 Q40280 1691 (Apple) 1.0201 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26545 Q9S7M5 1691 (Apple) 1.0202 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26547 Q9SYV3 1692 (Apple) 1.0203 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26548 Q9SYV4 1693 (Apple) 1.0204 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD26558 Q9SYV9 1694 (Apple) 1.0205 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAD13683 Q40280 1695 (Apple) 1.0206 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Ribonuclease-like PR-10a AAK13030 Q941P5 1696 (Apple) 1.0207 Malus domestica Mal d Yes Pathogenesis-related CAD32318 Q8L6K9 1697 (Apple) 1.0208 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related CAA96534 Q43549 1698 (Apple) 1.0301 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAK13027 Q941P8 1699 (Apple) 1.0302 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAK13028 Q941P7 1700 (Apple) 1.0303 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related AAO25113 Q84LA7 1701 (Apple) 1.0304 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related CAA96535 Q43550 1702 (Apple) 1.0401 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related CAA96536 Q43551 1703 (Apple) 1.0402 protein, PR-10, Bet v 1 family member Malus domestica Mal d Yes Pathogenesis-related CAA96537 Q43552 1704 (Apple) 1.0403 protein, PR-10, Bet v 1 family member Malus domestica Mal d 2 Yes Thaumatin-like protein AAC36740 Q9FSG7 1705 (Apple) Malus domestica Mal d Yes Non-specific lipid transfer AAT80637 Q5J026 1706 (Apple) 3.0101w protein type 1 Malus domestica Mal d Yes Non-specific lipid transfer AAT80649 Q5J011 1707 (Apple) 3.0102w protein type 1 Malus domestica Mal d Yes Non-specific lipid transfer AAT80656 Q5J009 1708 (Apple) 3.0201w protein type 1 Malus domestica Mal d Yes Non-specific lipid transfer AAT80664 Q5IZZ6 1709 (Apple) 3.0202w protein type 1 Malus domestica Mal d Yes Non-specific lipid transfer AAT80665 Q5IZZ5 1710 (Apple) 3.0203w protein type 1 Malus domestica Mal d Yes Profilin-3 AAD29414 Q9XF42 1711 (Apple) 4.0101 Malus domestica Mal d Yes Profilin (pf-3) CAD46561 Q84RR5 1712 (Apple) 4.0102 Malus domestica Mal d Yes Profilin-2 AAD29413 Q9XF41 1713 (Apple) 4.0201 Malus domestica Mal d Yes Profilin (pf-2) CAD46560 Q84RR6 1714 (Apple) 4.0202 Malus domestica Mal d Yes Profilin-1 AAD29412 Q9XF40 1715 (Apple) 4.0301 Malus domestica Mal d Yes Profilin (pf-1) CAD46559 Q84RR7 1716 (Apple) 4.0302 Manihot esculenta Man e 5 Yes Glutamic acid rich protein AEE98392 M1E7Y0 1717 (Cassava, manioc) Mercurialis annua Mer a 1 No Profilin CAA73720 O49894 1718 (Annual mercury) Morus nigra (Mulberry) Mor n 3 Yes Non-specific lipid transfer P85894 P85894 1719 protein type 1 Olea europaea (Olive) Ole e 1 No Common olive group 1 AAB32652 P19963 1720 Olea europaea (Olive) Ole e 2 No Profilin-1 CAA73035 O24169 1721 Olea europaea (Olive) Ole e 3 No Polcalcin AAD05375 O81092 1722 Olea europaea (Olive) Ole e 4 No major pollen allergen P80741 P80741 1723 Olea europaea (Olive) Ole e 5 No Superoxide dismutase [Cu—Zn] P80740 P80740 1724 Olea europaea (Olive) Ole e 6 No major pollen allergen AAB66909 O24172 1725 Olea europaea (Olive) Ole e 7 No putative non-specific lipid P81430 P81430 1726 transfer protein Olea europaea (Olive) Ole e 8 No Polcalcin-like protein (4 AAF31151 Q9M7R0 1727 EF-hands) Olea europaea (Olive) Ole e 9 No 1 3-beta glucanase AAK58515 Q94G86 1728 Olea europaea (Olive) Ole e 10 No X8 domain containing AAL92578 Q84V39 1729 protein Olea europaea (Olive) Ole e 11 No Pectin methylesterase ACZ57582 D8VPP5 1730 Ostrya carpinifolia Ost c 1 No Pathogenesis-related ADK39021 E2GL17 1731 (European protein, PR-10, Bet v 1 hophornbeam) family member Parietaria judaica Par j No Probable non-specific CAA54587 P43217 1732 (Pellitory-of-the-Wall) 1.0101 lipid-transfer protein Parietaria judaica Par j No Probable non-specific CAA65123 O04404 1733 (Pellitory-of-the-Wall) 1.0102 lipid-transfer protein 1 Parietaria judaica Par j No Probable non-specific CAI94601 Q1JTN5 1734 (Pellitory-of-the-Wall) 1.0103 lipid-transfer protein Parietaria judaica Par j No Probable non-specific CAA59370 Q40905 1735 (Pellitory-of-the-Wall) 1.0201 lipid-transfer protein 1 Parietaria judaica Par j No Phospholipid transfer CAA65121 P55958 1736 (Pellitory-of-the-Wall) 2.0101 protein Parietaria judaica Par j No Phospholipid transfer CAA65122 O04403 1737 (Pellitory-of-the-Wall) 2.0102 protein Parietaria judaica Par j No Profilin-1 CAB44256 Q9XG85 1738 (Pellitory-of-the-Wall) 3.0101 Parietaria judaica Par j No Profilin-2 CAB44257 Q9T0M8 1739 (Pellitory-of-the-Wall) 3.0102 Parietaria judaica Par j No Profilin CCP19647 L8BTD8 1740 (Pellitory-of-the-Wall) 3.0201 Parietaria judaica Par j 4 No Polcalcin CAP05019 B5QST3 1741 (Pellitory-of-the-Wall)

ietaria officinalis Par o 1 No Phospholipid transfer / / / (Pellitory) protein Parthenium Par h 1 No pollen defensin-like AKF12278 A0A0X9C7K4 1742 hysterophorus protein (Feverfew) Persea americana Pers a 1 Yes Endochitinase CAB01591 P93680 1743 (Avocado) Phaseolus vulgaris Pha v Yes non-specific lipid transfer ADC80502 D3W146 1744 (Green bean, French 3.0101 protein type 1 bean) Phaseolus vulgaris Pha v Yes non-specific lipid transfer ADC80503 D3W147 1745 (Green bean, French 3.0201 protein type 1 bean) Pistacia vera (Pistachio) Pis v 1 Yes 2S albumin ABG73108 B7P072 1746 Pistacia vera (Pistachio) Pis v Yes 11S globulin subunit ABG73109 B7P073 1747 2.0101 presucor Pistacia vera (Pistachio) Pis v Yes 11S globulin subunit ABG73110 B7P074 1748 2.0201 presucor Pistacia vera (Pistachio) Pis v 3 Yes vicillin ABO36677 B4X640 1749 Pistacia vera (Pistachio) Pis v 4 Yes manganese superoxide ABR29644 B2BDZ8 1750 dismutase Pistacia vera (Pistachio) Pis v 5 Yes 11S globulin subunit ACB55490 B7SLJ1 1751 Pisum sativum (Pea) Pis s Yes Vicilin CAF25232 Q702P1 1752 1.0101 Pisum sativum (Pea) Pis s Yes Vicilin CAF25233 Q702P0 1753 1.0102 Pisum sativum (Pea) Pis s 2 Yes Convicilin CAB82855 P13915 1754 Pisum sativum (Pea) Pis s 3 Yes Non-specific lipid-transfer AJG44053 C0HJR7 1755 protein 1 Plantago lanceolata Pla l No Ole e 1-related protein CAC41633 P82242 1756 (English plantain) 1.0101 Plantago lanceolata Pla l No Ole e 1-related protein CAC41634 P82242 1756 (English plantain) 1.0102 (variant D58G) Plantago lanceolata Pla l No Ole e 1-related protein CAC41635 P82242 1756 (English plantain) 1.0103 (variant D58G S82G) Plantago lanceolata Pla l 2 No Profilin / C0HJX6 1757 (English plantain) Platanus acerifolia Pla a 1 No Putative invertase inhibitor CAD20556 Q8GT41 1758 (London plane tree) Platanus acerifolia Pla a 2 No Polygalacturonase CAE52833 Q6H9K0 1759 (London plane tree) Platanus acerifolia Pla a 3 No Non-specific lipid transfer / / / (London plane tree) protein 1 Platanus orientalis Pla or 1 No Plant invertase/pectin ABY21305 A9YUH4 1760 (Oriental plane) methylesterase inhibitor Platanus orientalis Pla or 2 No Polygalacturonase ABY21306 A9YUH5 1761 (Oriental plane) Platanus orientalis Pla or 3 No Non-specific lipid-transfer ABY21307 A9YUH6 1762 (Oriental plane) protein 1 Prosopis juliflora Pro j 1 No Ole e 1-like protein AKV72167.1 / 1763 (Mesquite) Prosopis juliflora Pro j 2 No Profilin AHY24177 A0A023W2L7 1764 (Mesquite) Prunus armeniaca Pru ar 1 Yes Pathogenesis-related AAB97141 O50001 1765 (Apricot) protein, PR-10, Bet v 1 family member Prunus armeniaca Pru ar 3 Yes Non-specific lipid transfer P81651 P81651 1766 (Apricot) protein 1 Prunus avium (Sweet Pru av Yes Pathogenesis-related AAC02632 O24248 1767 cherry) 1.0101 protein, PR-10, Bet v 1 family member Prunus avium (Sweet Pru av Yes Pathogenesis-related AAS47035 Q6QHU3 1768 cherry) 1.0201 protein, PR-10, Bet v 1 family member Prunus avium (Sweet Pru av Yes Pathogenesis-related AAS47036 Q6QHU2 1769 cherry) 1.0202 protein, PR-10, Bet v 1 family member Prunus avium (Sweet Pru av Yes Pathogenesis-related AAS47037 Q6QHU1 1770 cherry) 1.0203 protein, PR-10, Bet v 1 family member Prunus avium (Sweet Pru av 2 Yes Thaumatin-like protein AAB38064 P50694 1771 cherry) Prunus avium (Sweet Pru av 3 Yes Non-specific lipid transfer AAF26449 Q9M5X8 1772 cherry) protein 1 (nsLTP1) Prunus avium (Sweet Pru av 4 Yes Profilin AAD29411 Q9XF39 1773 cherry) Prunus domestica Pru d 3 Yes Non-specific lipid transfer P82534 P82534 1774 (European plum) protein 1 (nsLTP1) Prunus dulcis (Almond) Pru du 3 Yes Non-specific lipid transfer ACN11576 C0L0I5 1775 protein 1 (nsLTP1) Prunus dulcis (Almond) Pru du 4 Yes Profilin AAL91662 Q8GSL5 1776 Prunus dulcis (Almond) Pru du 5 Yes 60s acidic ribosomal prot. ABH03379 Q8H2B9 1777 P2 Prunus dulcis (Almond) Pru du Yes Prunin-1 (Amandin, 11S ADN39440 E3SH28 1778 6.0101 globulin legumin-like protein) Prunus dulcis (Almond) Pru du Yes Prunin-2 ADN39441 E3SH29 1779 6.0201 Prunus mume (Japanese Pru m 7 Yes gibberellin-regulated XP_016648029.1 / 1780 apricot) protein Prunus persica (Peach) Pru p 1 Yes Pathogenesis-related ABB78006 Q2I6V8 1781 protein, PR-10, Bet v 1 family member Prunus persica (Peach) Pru p Yes Thaumatin-like protein ACE80959 B6CQT7 1782 2.0101 Prunus persica (Peach) Pru p Yes Thaumatin-like protein ACE80957 B6CQT5 1783 2.0201 Prunus persica (Peach) Pru p Yes Thaumatin-like protein ACE80955 B6CQT3 1784 2.0301 Prunus persica (Peach) Pru p Yes Non-specific lipid transfer P81402 P81402 1785 3.0101 protein 1 (nsLTP1) Prunus persica (Peach) Pru p Yes Non-specific lipid transfer CAB96876 Q9LED1 1786 3.0102 protein 1 (nsLTP1) Prunus persica (Peach) Pru p 4 Yes Profilin CAD37201 Q8GT40 1787 Prunus persica (Peach) Pru p 7 Yes Gibberellin-regulated P86888 P86888 1788 protein Punica granatum Pun g Yes Non-specific lipid transfer AHB19227 A0A059STC4 1789 (Pomegranate) 1.0101 protein 1 (nsLTP1) Punica granatum Pun g Yes Non-specific lipid transfer AHB19226 A0A059SSZ0 1790 (Pomegranate) 1.0201 protein 1 (nsLTP1) Punica granatum Pun g Yes Non-specific lipid transfer AHB19225 A0A059ST23 1791 (Pomegranate) 1.0301 protein 1 (nsLTP1) Pyrus communis (Pear) Pyr c 1 Yes Pathogenesis-related AAC13315 O65200 1792 protein, PR-10, Bet v 1 family member Pyrus communis (Pear) Pyr c 3 Yes Nonspecific lipid-transfer AAF26451 Q9M5X6 1793 protein 1 Pyrus communis (Pear) Pyr c 4 Yes Profilin AAD29410 Q9XF38 1794 Pyrus communis (Pear) Pyr c 5 Yes Isoflavone reductase AAC24001 O81355 1795 related protein, putative phenylcoumaran benzylic ether reductase Quercus alba (White Que a No Pathogenesis-related ABZ81045 B6RQS1 1796 oak) 1.0201 protein, PR-10, Bet v 1 family member Quercus alba (White Que a No Pathogenesis-related ABZ81046 B6RQS2 1797 oak) 1.0301 protein, PR-10, Bet v 1 family member Quercus alba (White Que a No Pathogenesis-related ABZ81047 B6RQS3 1798 oak) 1.0401 protein, PR-10, Bet v 1 family member Ricinus communis Ric c 1 Yes 2S albumin CAA38097 P01089 1799 (Castor bean) Rubus idaeus (Red Rub i 1 Yes Pathogenesis-related ABG54495 Q0Z8U9 1800 raspberry) protein, PR-10, Bet v 1 family member Rubus idaeus (Red Rub i 3 Yes Non-specific lipid transfer ABG54494 Q0Z8V0 1801 raspberry) protein 1 (nsLTP1) Salsola kali (Russian Sal k No Pectin methylesterase P83181 P83181 1802 thistle, Saltwort) 1.0101 Salsola kali (Russian Sal k No Pectinesterase AAT99258 I6LD58 1803 thistle, Saltwort) 1.0201 Salsola kali (Russian Sal k No Pectinesterase AAX11262 Q17ST3 1804 thistle, Saltwort) 1.0301 Salsola kali (Russian Sal k No Pectinesterase AAX11261 Q17ST4 1805 thistle, Saltwort) 1.0302 Salsola kali (Russian Sal k 2 No Protein kinase homologue AAN05083 Q8L5K9 1806 thistle, Saltwort) Salsola kali (Russian Sal k 3 No Cobalamin independent ACO34814 C1KEU0 1807 thistle, Saltwort) methionine synthase Salsola kali (Russian Sal k No Profilin ACS34771 C6JWH0 1808 thistle, Saltwort) 4.0101 Salsola kali (Russian Sal k No Profilin ADK22841 E2D0Y9 1809 thistle, Saltwort) 4.0201 Salsola kali (Russian Sal k 5 No Ole e 1-like protein ADK22842 E2D0Z0 1810 thistle, Saltwort) Sesamum indicum Ses i 1 Yes 2S albumin AAK15088 Q9AUD1 1811 (Sesame) Sesamum indicum Ses i 2 Yes 2S seed storage protein 1 AAD42943 Q9XHP1 1812 (Sesame) Sesamum indicum Ses i 3 Yes 7S vicilin-like globulin AAK15089 Q9AUD0 1813 (Sesame) Sesamum indicum Ses i 4 Yes oleosin AAG23840 Q9FUJ9 1814 (Sesame) Sesamum indicum Ses i 5 Yes oleosin AAD42942 Q9XHP2 1815 (Sesame) Sesamum indicum Ses i 6 Yes 11S globulin seed storage AAD42944 Q9XHP0 1816 (Sesame) protein 2 Sesamum indicum Ses i 7 Yes 11S globulin AAK15087 Q9AUD2 1817 (Sesame) Sinapis alba (Yellow Sin a 1 Yes 2S albumin CAA62909 P15322 1818 mustard) Sinapis alba (Yellow Sin a 2 Yes 11S globulin (legumin- AAX77383 Q2TLW0 1819 mustard) like) seed storage protein Sinapis alba (Yellow Sin a 3 Yes non-specific lipid transfer ABU95411 E6Y2L9 1820 mustard) protein type 1 Sinapis alba (Yellow Sin a 4 Yes Profilin ABU95412 E6Y2M0 1821 mustard) Solanum lycopersicum Sola l 1 Yes Profilin-2 CAD10377 Q93YG7 1822 (Lycopersicon esculentum) (Tomato) Solanum lycopersicum Sola l Yes Beta-fructofuranosidase AAL75449 Q547Q0 1823 (Lycopersicon 2.0101 esculentum) (Tomato) Solanum lycopersicum Sola l Yes Beta-fructofuranosidase AAL75450 Q8RVW4 1824 (Lycopersicon 2.0201 esculentum) (Tomato) Solanum lycopersicum Sola l 3 Yes Non-specific lipid-transfer AAB42069 P93224 1825 (Lycopersicon protein 2 esculentum) (Tomato) Solanum lycopersicum Sola l Yes Pathogenesis-related AHC08073 K4CWC5 1826 (Lycopersicon 4.0101 protein, PR-10, Bet v 1 esculentum) (Tomato) family member, TSI-1 Solanum lycopersicum Sola l Yes Pathogenesis-related NP_001275580 K4CWC4 1827 (Lycopersicon 4.0201 protein, PR-10, Bet v 1 esculentum) (Tomato) family member, TSI-1 Solanum lycopersicum Sola l 5 Yes Cyclophilin (Peptidyl- AAA63543 P21568 1828 (Lycopersicon prolyl cis-trans isomerase) esculentum) (Tomato) Solanum lycopersicum Sola l 6 Yes Non-specific lipid transfer XP_004232333 K4BBD9 1829 (Lycopersicon protein type 2 (nsLTP2) esculentum) (Tomato) Solanum lycopersicum Sola l 7 Yes nsLTP type 1 / / / (Lycopersicon esculentum) (Tomato) Solanum tuberosum Sola t 1 Yes Patatin CAA31576 P15476 1830 (Potato) Solanum tuberosum Sola t 2 Yes Cathepsin D inhibitor PDI P16348 P16348 1831 (Potato) Solanum tuberosum Sola t Yes Cysteine protease inhibitor AAB63099 O24383 1832 (Potato) 3.0101 10 Solanum tuberosum Sola t Yes Cysteine protease inhibitor AAA33845 P20347 1833 (Potato) 3.0102 1 Solanum tuberosum Sola t 4 Yes Serine protease inhibitor 7 BAA04149 P30941 1834 (Potato) Syringa vulgaris (Lilac) Syr v No Ole e 1-related protein, S43243 / 1835 1.0102 isoform 2 Syringa vulgaris (Lilac) Syr v No Olee 1-related protein, S43244 / 1836 1.0103 isoform 3 Syringa vulgaris (Lilac) Syr v 3 No Polcalcin AAK01144 P58171 1837 Triplochiton Trip s 1 No Endochitinase / C0HJM6 1838 scleroxylon (Obeche) Vigna radiata (Mung Vig r 1 Yes Pathogenesis-related AAX19889 Q2VU97 1839 bean) protein, PR-10, Bet v 1 family member Vigna radiata (Mung Vig r Yes 8S Globulin (Vicilin), beta ABG02262 Q198W3 1840 bean) 2.0101 isoform Vigna radiata (Mung Vig r Yes 8S globulin alpha subunit ABW23574 B1NPN8 1841 bean) 2.0201 Vigna radiata (Mung Vig r 4 Yes Seed albumin CAA50008 Q43680 1842 bean) Vigna radiata (Mung Vig r 6 Yes Cytokinin-specific binding BAA74451 Q9ZWP8 1843 bean) protein (CSBP), Bet v 1 family member Vitis vinifera (Grape) Vit v 1 Yes Non-specific lipid transfer AAO33394 Q850K5 1844 protein 1 (nsLTP1) Ziziphus mauritiana Ziz m 1 Yes Class III chitinase AAX40948 Q2VST0 1845 (Chinese-date) Plantae Pinopsida Chamaecyparis obtusa Cha o 1 No Pectate lyase BAA08246 Q96385 1846 (Japanese cypress) Chamaecyparis obtusa Cha o 2 No Polygalacturonase Q7M1E7 Q7M1E7 1847 (Japanese cypress) Chamaecyparis obtusa Cha o 3 No Cellulase (glycosyl / / / (Japanese cypress) hydrolase) Cryptomeria japonica Cry j No Pectate lyase BAA05542 P18632 1848 (Sugi) 1.0101 Cryptomeria japonica Cry j No Pectate lyase BAB86286 Q8RUR1 1849 (Sugi) 1.0103 Cryptomeria japonica Cry j 2 No Polygalacturonase / / / (Sugi) Cupressus arizonica Cup a 1 No Pectate lyase BAA06172 P43212 1850 (Cypress) Cupressus Cup s No Pectate lyase AAF72625 Q9M4S6 1851 sempervirens (Common 1.0101 cypress) Cupressus Cup s No Pectate lyase AAF72626 Q9M4S5 1852 sempervirens (Common 1.0102 cypress) Cupressus Cup s No Pectate lyase AAF72627 Q9M4S4 1853 sempervirens (Common 1.0103 cypress) Cupressus Cup s No Pectate lyase AAF72628 Q9M4S3 1854 sempervirens (Common 1.0104 cypress) Cupressus Cup s No Pectate lyase AAF72629 Q9M4S2 1855 sempervirens (Common 1.0105 cypress) Cupressus Cup s 2 No Polygalacturonase / C0HKB1 1856 sempervirens (Common cypress) Cupressus Cup s No Thaumatin-like protein AAR21073 Q69CS2 1857 sempervirens (Common 3.0101 cypress) Cupressus Cup s No Thaumatin-like protein AAR21074 Q69CS3 1858 sempervirens (Common 3.0102 cypress) Juniperus ashei Jun a No Pectate lyase AAD03608 P81294 1859 (Mountain cedar) 1.010101 Juniperus ashei Jun a No Pectate lyase AAD03609 P81294 1859 (Mountain cedar) 1.010102 Juniperus ashei Jun a 2 No Polygalacturonase CAC05582 Q9FY19 1860 (Mountain cedar) Juniperus ashei Jun a 3 No Thaumatin-like protein AAF31759 P81295 1861 (Mountain cedar) Juniperus oxycedrus Jun o 4 No Polcalcin-like protein (4 AAC15474 O64943 1862 (Prickly juniper) EF hand domains) Juniperus sabinoides Jun s 1 No / / / / (Mountain cedar) Juniperus virginiana Jun v No Pectate lyase-1 AAF80166 Q9LLT2 1863 (Eastern red cedar) 1.0101 Juniperus virginiana Jun v No Pectate lyase-1 AAF80164 Q9LLT1 1863 (Eastern red cedar) 1.0102 Juniperus virginiana Jun v 3 No Thaumatin-like protein AAF80167 Q9LD79 1864 (Eastern red cedar) Pinus koraiensis Pin k 2 No Vicilin AHC94918 V9VGU0 1865 (Korean Pine) Pinus pinea (Stone Pin p 1 No 2S albumin CTQ87571.1 / 1866 pine)

indicates data missing or illegible when filed

In some embodiments, SPNs, magnetic particle conjugates and compositions of the present invention may detect a specific epitope of a target allergen. As used herein, an “epitope” is the part of the allergen that is recognized by the immune system (e.g., antibodies. B cells, or T cells). Generally, the whole allergen is not involved in the immune response, but rather, the epitopes of allergens, which are recognized by a T-cell receptor or an IgE-antibody, contribute to allergic reactions. SPNs, magnetic particle conjugates and compositions of the present invention may bind to an epitope of a target allergen in a similar manner as antibodies or T-cell receptors.

Epitopes of an allergen protein may be identified using methods and techniques known in the art. For example, IgE-binding epitopes may be determined by methods such as X-ray co-crystallography of allergens and immunocomplexes, array-based oligo-peptide scanning, mutagenesis mapping, or nuclear magnetic resonance. For example, T-cell epitopes may be identified using short peptide fragments that overlap the entire amino acid sequence of the target allergen and allergen-specific T-cell lines derived from peripheral blood mononuclear cells. Peptides that induce T-cell proliferation contain T-cell epitopes. Additional techniques that may be used to determine epitopes on an allergen protein include crosslinking coupled mass spectrometry, hydrogen-deuterium exchange, and computer-based in silico analysis. Many epitopes of common food allergens have been identified, such as those listed in Tables 1-5 of Matsuo H et al., Allergol Int. 2015 October; 64(4):332-43.

In some embodiments, SPNs, magnetic particle conjugates and compositions of the present invention may be used in a hospital for clinical food allergy or allergy test and to identify food/allergen(s) to which a patient is allergic. In addition, SPNs, magnetic particle conjugates and compositions of the present invention may be used as a carry-on tester for people who have food/environmental allergy, for example at home to test commercial food, or at restaurant to check dishes they ordered. The food sample could be fresh food, frozen food, cooled food or processed food containing animal derived meat and/or vegetables.

In some embodiments, SPNs, magnetic particle conjugates and compositions of the present invention may detect other target molecules, including but not limited to, pathogens from a pathogenic microorganism in a sample, such as bacteria, yeasts, fungi, spores, viruses or prions; disease proteins (e.g., biomarkers for diseases diagnosis and prognosis); pesticides and fertilizers remained in the environment; and toxins. In other embodiments, SPNs and compositions of the present invention may bind to non-protein targets such as minerals and small molecules (e.g., antibiotics), drugs and inorganic ion.

II. Kits, Packaging and Biosensors

Compositions, SPNs, SPN-complement complexes, magnetic particle conjugates, DNA-printed solid substrates and detection agents of the present invention may be combined with other ingredients or reagents or prepared as components of kits or other retail products for commercial sale or distribution.

The kit will contain compositions of the present invention, along with instructions regarding administration and/or use of the kit. The kit may also contain one or more of the following: a syringe, a bag or bottle.

Formulations and/or compositions of the present invention can be packaged for use in a variety of pharmaceutically or diagnostically acceptable containers using any acceptable container closure, as the formulations are compatible with PVC-containing and PVC-free containers and container closures. Examples of acceptable containers include, but are not limited to, ampules and pre-filled syringes, cartridges and the like.

Alternatively, the formulation may contain SPNs, SPN-complement complexes, magnetic particle conjugates in one compartment of an admix bag and an acceptable solvent in a separate compartment of the admix bag such that the two compartments may be mixed together prior to use. Acceptable containers are well known in the art and commercially available.

In some embodiments, biosensors comprising compositions, SPN-complement complexes, magnetic particle conjugates, DNA-printed solid substrates and detection agents of the present invention are provided. The biosensor may be an on-chip magnetic particle biosensor. For example, a plurality of magnetic particle sensors are embedded in the integrated circuit; the magnetic particle sensors are capable of detecting magnetic particles specifically bound to the one or more sensor areas on the surface of the integrated circuit. The affinity molecules on the surface of the sensor area may be SPNs, or SPN-complement complexes of the present invention.

In some embodiments, a graphene-oxide (GO) based biosensor is provided, wherein the sensing agents are SPNs conjugated to the graphene-oxide surface.

In some aspects, it may be a “signal on” biosensor. The SPN and its complementary sequence may be labeled with a fluorophore and a quencher at one end of the nucleic acid sequence, respectively. The signal produced by the sensor is dependent on the structural changes in the SPNs following the binding of target allergens. The binding of the target allergen to the SPN disrupts the SPN-complement complex and replaces the complementary sequence in the complex, resulting in the quenched fluorescent signal back on (FIG. 4B).

In some aspects, it may be a “signal off” biosensor, in which the complementary sequence is labeled with a fluorophore at one end of the sequence. The binding of the target allergen to the SPN detaches the complementary sequence in the complex, causing the fluorescent signal off (FIG. 4A).

In other aspects, it may be a “dual signal” biosensor, in which the SPN and the complementary sequence are labeled with different fluorophores. The competition between the target allergen and the complement will change the fluorescent signals (FIG. 4C).

III. Detection Methods and Assays

In accordance with the present invention, aptamers, SPNs and SPN-complement complexes, magnetic particle conjugates, DNA-printed solid substrates, detection agents and compositions of the present invention may be used to, in a broad concept, detect any molecules in a sample in a large variety of applications, such as food safety, diagnostic and prognostic tests in civilian and battlefield settings, environmental monitoring/control, and military use for detection of biological weapons. Various methods and assays may be used in combination with aptamers, SPNs, SPN-complement complexes, magnetic particle conjugates, DNA-printed solid substrates, detection agents and compositions of the present invention, the choice may depend on the application field.

Particularly the present invention provides methods of determining the absence, presence and/or quantity of one or more target allergens in a sample using detection agents comprising SPN-magnetic particle conjugates and printed solid substrates. In some embodiments, the detection assays and methods can be used in a hospital for clinical food allergy or allergy test and to identify food/allergen(s) to which a patient is allergic. Such assays and methods may be used to monitor allergen contamination in food industry. Additionally, they may also be used at home or in a restaurant by a person who has allergy to test the allergen content before he/she consumes the food.

Examples of foods are eggs, milk, meat, fishes, crustacea and mollusks, cereals, legumes and nuts, fruits, vegetables, beer yeast, and gelatin; more particularly, egg white and egg yolk of the eggs, milk and cheese of the milk, pork, beef, chicken and mutton of the meat, mackerel, horse mackerel, sardine, tuna, salmon, codfish, flatfish and salmon caviar of the fishes, crab, shrimp, blue mussel, squid, octopus, lobster and abalone of the crustacea and mollusks, wheat, rice, buckwheat, rye, barley, oat, corn, millet, foxtail millet and barnyardgrass of the cereals, soybean, peanut, cacao, pea, kidney bean, hazelnut, Brazil nut, almond, coconut and walnut of the legumes and nuts, apple, banana, orange, peach, kiwi, strawberry, melon, avocado, grapefruit, mango, pear, sesame and mustard of the fruits, tomato, carrot, potato, spinach, onion, garlic, bamboo shoot, pumpkin, sweet potato, celery, parsley, yam and Matsutake mushroom of the vegetables, the foods containing them, and the ingredients thereof (e.g., ovoalbumin, ovomucoid, lysozyme, casein, beta-lactoglobulin, alpha-lactoalbumin, gluten, and alpha-amylase inhibitor).

The foods could be fresh foods, frozen foods, cooled foods or processed foods containing animal derived meat and/or vegetables. These foods may be processed by heating, freezing, drying, salting, fermentation, enzymatic processing, etc.

In some embodiments, more than one agents may be used, depending on the nature of the food matrixes. Some food contains several allergenic proteins, e.g., at least eight peanut proteins, such as Ara h1 and Ara h2, can potentially cause an immunological response. In such case, more than one SPNs against more than one allergenic protein may be used in a mixed cocktail for detecting the absence or presence of peanut. In other aspects, some food matrixes such as fish, shellfish and mollusks, contain only one major allergenic protein. One or more SPNs that specifically bind to this major allergen protein may be used for allergen detection.

In some embodiments, allergen detection assays and methods of the present invention can detect a lower concentration of allergen in a food sample. The sensitivity of nucleic acid aptamers makes it possible to detect the presence of an allergen as low as 0.0001 ppm. In some aspects, the concentration or mass of allergen that can be detected may range from 0.001 ppm to 5 ppm, or from 0.001 ppm to 0.1 ppm, or from 0.1 ppm to 3 ppm, or from 1 ppm to 5 ppm, or from 5 ppm to 10 ppm, or from 10 ppm to 50 ppm, or from 10 ppm to 20 ppm, or from 10 ppm to 100 ppm. In some aspects, the concentration or mass of allergen in a food sample that can be detected may be 0.001 ppm, 0.002 ppm, 0.003 ppm, 0.004 ppm, 0.005 ppm, 0.006 ppm, 0.007 ppm, 0.008 ppm, 0.009 ppm, 0.01 ppm, 0.02 ppm, 0.03 ppm, 0.04 ppm, 0.05 ppm, 0.06 ppm, 0.07 ppm, 0.08 ppm, 0.09 ppm, 0.1 ppm, 0.2 ppm, 0.3 ppm, 0.4 ppm, 0.5 ppm, 0.6 ppm, 0.7 ppm, 0.8 ppm, 0.9 ppm, 1.0 ppm, 1.5 ppm, 2 ppm, 2.5 ppm, 3 ppm, 3.5 ppm, 4 ppm, 4.5 ppm, 5 ppm or 10 ppm. In some embodiments, the concentration or mass of allergen in a food sample that can be detected may be 5 ppm, 1 ppm, 15 ppm, 20 ppm, 25 ppm, 30 ppm, 35 ppm, 40 ppm, 45 ppm, 50 ppm, 55 ppm, 60 ppm, 65 ppm, 70 ppm, 75 ppm, 80 ppm, 85 ppm, 90 ppm, 95 ppm or 100 ppm. In one embodiment, the concentration or mass of allergen in a food sample that can be detected may be at low as 50 ppm. In another embodiment, the concentration or mass of allergen in a food sample that can be detected may be at low as 12.5 ppm

In accordance with the present aptamer derived SPN based detection assays, the sensitivity can be achieved regardless of food matrices. The diverse food matrices with different salt, fat and sugar content, different color, texture, and pH can be detected at the present sensitivity.

In some embodiments, methods of the present invention for detecting the absence, presence and/or quantity of a target allergen in a test sample comprise (a). obtaining and processing a test sample which is suspected to contain an allergen of interest; (b). contacting the processed test sample with detection agents comprising SPNs conjugated to solid substrates, wherein the SPNs are single-stranded nucleic acid molecules having 20 to 200 nucleotides capable of specifically binding to the target allergen; (c) washing the mixture of the detection agents and the test sample formed in step (b); (d). detecting the allergen-SPN complexes formed during the assay; and (e). processing and analyzing the detection signals to determine whether the target allergen is present in the food sample and/or the quantity of the target allergen in the sample.

In some aspects, the detection agents further comprise a nucleic acid molecule complementary to a region of the SPN sequence which binds to the SPN only when the SPN is not bound to its target allergen protein; the SPN and the complementary sequence forms the SPN-complement complex, in which the SPN and the complementary sequence work as binding ligand (to the target allergen) and detection molecule or label, respectively. In some examples, the SPN is covalently immobilized on the surface of the solid substrate through its 5′end or 3′end. In other examples, the complementary sequence is covalently immobilized on the surface of the solid substrate.

In some examples, the solid substrate is magnetic particles. In accordance, the magnetic particles may be held using a magnetic field during the wash step. Optionally, the washed reaction mixture may be shaken, prior to detecting the allergen-SPN-magnetic particle complexes formed during the assay.

Assays and methods of the present invention may have various forms depending on biosensors, detection kits and detection devices and systems used to implement the assays. SPN/complement-magnetic particle conjugates may be used in any steps of the assays, such as capture agents to capture a target analyte (e.g., a target allergen or a specific epitope of the target allergen) in a sample; or detector agents for signaling detection; or competitive binding agents, or affinity agents to selected a target analyte (e.g., an allergen) bound magnetic particles.

In some embodiments, SPNs comprise the nucleic acid sequences of SEQ ID NOs.: 1-696 (See Tables 1-4). The complementary sequences may contain about 5-20 nucleotide residues. The SPN and its complementary sequence may be at a ratio of 1:5, or at a ratio of 1:4, or at a ratio of 1:3, or at a ratio of 1:2.

In some embodiments, an attachment assay may be developed using the compositions and agents of the present invention (as shown in FIG. 6A). Accordingly, the assay may comprise steps of (a). obtaining and processing a test sample which is suspected to contain an allergen of interest; (b). contacting the processed sample with signaling polynucleotides (SPNs) which specifically bind to the allergen of interest, wherein the SPNs are labeled with a fluorophore at one end of the sequence; (c). exposing the mixture of the processed sample and the SPNs formed in step (b) to the surface of a solid substrate, wherein the surface of the solid substrate comprises nucleic acid sequences that are complementary to a region of the SPN sequence; (d). washing the mixture formed in step (c); (e). detecting a fluorescent signal from the surface of the solid substrate; and (f). processing and analyzing the fluorescent signal to determine the absence, presence, and/or the quantity of the allergen of interest in the test sample. The free SPNs which are not bound to the allergen proteins will bind to the complementary sequences printed on the solid surface and will contribute to the fluorescence reading, while the SPNs which are bound to the allergen proteins will not attach to the solid surface and will be washed away. The fluorescence reading will indicate the absence, presence or quantity of the allergen of interest in the test sample.

In other embodiments, a detachment assay may be developed using the compositions and agents of the present invention (as shown in FIG. 6B). Accordingly, the assay may comprise steps of (a) obtaining and processing a test sample which is suspected to contain an allergen of interest; (b) exposing the processed sample to the surface of a solid substrate, wherein the surface of the solid substrate comprises SPN-complement complexes which specifically bind the allergen of interest; (c) washing the mixture formed in step (b); (d) detecting a fluorescent signal from the surface of the solid substrate and comparing the fluorescent signal to that detected prior to the exposure of the processed sample; and (e) processing and analyzing the fluorescent signal to determine the absence, presence, and/or the quantity of the allergen of interest in the test sample. In accordance with this detachment assay, the SPN complementary sequences are printed to the surface of the solid substrate. The SPNs which specifically bind to the allergen of interest are incubated with the surface. The mixture will be washed and a fluorescence reading is recorded. The allergen proteins in the test sample, when added to the SPN-complement complexes, will bind to the SPNs and the SPN-protein complexes detach from the complementary sequences and will be washed away. The fluorescence reading from step (d) is compared with the preread fluorescence signal; the difference may be used for determining the absence, presence or quantity of the allergen of interest in the test sample.

In some embodiments, SPNs with different sequences but having a high affinity and specificity to the same target allergen may be used in combination. In other aspects, SPNs of the present invention may be used in combination with antibodies that bind the same target allergen in a detection assay.

In some embodiments, the detection assay of the present invention can be optimized depending on the testing condition such as food matrix. The reaction buffer used may be decreased in volume. In some aspects. The reaction volume can be limited to less than 5 mL, for example, less than 4 mL, or less than 3 mL, or less than 2 mL, or less than 1 mL. In one example, the volume may be 1.5 mL, 2 mL, 2.5 mL, 3 mL, 3.5 mL, 4.5 mL, and 5.0 mL.

In some embodiments, the sample size can be reduced, limiting the requirement of a large size sample. The assay sensitivity can be achieved with a small portion of test sample, for example, less than 5 mg, or less than 4.5 mg, or less than 4 mg, or less than 3.5 mg, or less than 3 mg, or less than 2.5 mg, or less than 2 mg, or less than 1.5 mg.

In some embodiments, the detection assay of the present invention can be completed in a short period of time, for example less than 5 minutes. In some aspects, the detection reaction can be completed from 10 seconds to 5 minutes, or from 10 seconds to 60 seconds, or from 1 minute to 2 minutes. In some examples, the detection assay can be completed in about 10 seconds, about 20 seconds, about 30 seconds, about 35 seconds, about 40 seconds, about 45 seconds, about 50 seconds, about 1 minute, about 1.5 minutes, about 2 minutes, about 2.5 minutes, about 3 minutes, about 4.5 minutes, or about 5 minutes.

In some embodiments, the detection assays of the present invention can be optimized to achieve the greatest signal intensity. The step optimization may include, but are not limited to, changing the concentration of SPN molecules, controlling the sample and SPN incubation conditions and time, controlling the flow rate and maximizing the exposure of solid surface to SPNs.

In some embodiments, the detection assay of the present invention further comprising an internal control signal. The built-in control signal may be measured using pre-incubated free SPNs and/or free food samples without SPN binding. These control signals will reduce the background signal and non-specific reading during the detection reaction.

In some embodiments, the detection signals are processed and displayed by a reader device. The reader device may be a computer, an iPad and/or a cellphone, or other processors that can execute one or more methods for detecting the absence, presence and/or quantity of the target allergen.

In accordance with the present invention, the detection agents and other reaction agents of the detection assay are stable and can be stored for a long-period of time. In general, short nucleic acid molecules are stable at routine storage condition. In some aspects, the SPNs, SPN-magnetic bead conjugates and nucleic acid coated solid surfaces are stable and can maintain their activity for at least one month, or at least two months, or at least three months, or at least four months, or at least five months, or at least six months. They may be stable from about one month to about one year. The reaction agents such as the extraction buffer can be stable at various temperature for at least nine months, or at least ten months, or at least one year.

IV. Definitions

At various places in the present specification, substituents of compounds of the present disclosure are disclosed in groups or in ranges. It is specifically intended that the present disclosure include each and every individual sub-combination of the members of such groups and ranges. The following is a non-limiting list of term definitions.

Activity: As used herein, the term “activity” refers to the condition in which things are happening or being done. Compositions of the invention may have activity and this activity may involve the binding to a target molecule.

Allergen: as used herein, the term “allergen” means a compound, substance or composition that causes, elicits or triggers and immune reaction in a subject. As such, allergens are typically referred to as antigens. An allergen is typically a protein or a polypeptide.

Allergen detection agent: As used herein, the term “an allergen detection agent” refers to Any agent which is capable of, or does, interact with and/or bind to one or more allergens in a way that allows detection of such allergen in a sample is referred to herein as an “allergen detection agent” or “detection agent”.

Analyte: As used herein, an “analyte” is a target of interest that can specifically interact with (bind to) an aptamer and be detected and/or measured. In the context of the present invention, an analyte may be an allergen.

Aptamer: as used herein, the term“aptamer” refers to single stranded nucleic acid. In general, aptamers refer to either an oligonucleotide of a single defined sequence or a mixture of said oligonucleotides, wherein the mixture retains the properties of binding specifically to a target allergen. A RNA aptamer is an aptamer comprising ribonucleoside units. RNA aptamer also meant to encompass RNA analogs as defined herein. A DNA aptamer an aptamer comprising deoxy-ribonucleoside units. DNA aptamer also meant to encompass DNA analogs as defined herein.

Binding affinity: as used herein, the term “binding affinity” is intended to refer to the tendency of an aptamer to bind or not bind a target and describes the measure of the strength of the binding or affinity of the aptamer to bind the target.

Complementary: As used herein, the term “complementary” or “complement” refer to the natural binding of polynucleotides by base pairing such as A-T(U) and C-G pairs. Two single-stranded molecules may be partially complementary such that only some of the nucleic acids bind, or it may be “complete,” such that total complementarity exists between the single stranded molecules. The degree of complementarity between nucleic acid strands has significant effects on the efficiency and strength of the hybridization between the nucleic acid strands.

Detection: As used herein, the term “detection” means an extraction of a particular target protein from a mixture of many non-target proteins, indicating the absence, presence, and/or amount of a target protein from a mixture of many non-target proteins.

Hybridization: As used herein, the term “hybridization” refers to the process by which a polynucleotide strand anneals with a complementary strand through base pairing under defined hybridization conditions. Specific hybridization is an indication that two nucleic acid sequences share a high degree of identity such as a SPN of the present invention and a short complementary sequence of the SPN. Specific hybridization complexes form under permissive annealing conditions and remain hybridized after the “washing” step(s). The washing step(s) is particularly important in determining the stringency of the hybridization process, with more stringent conditions allowing less non-specific binding. i.e., binding between pairs of nucleic acid strands that are not perfectly matched.

Magnetic particles: As used herein, the term “magnetic particles” refer to ( ). Magnetic particles may include magnetic microbeads and/or nanoparticles.

Oligonucleotide: as used herein, the term “oligonucleotide” is generic to polydeoxyribonucleotides (containing 2′-deoxy-D-ribose or modified forms thereof), i.e. DNA, to polyribonucleotides (containing D ribose or modified forms thereof), i.e. RNA, and to any other type of polynucleotide which is an N-glycoside or C-glycoside of a purine or pyrimidine base, or modified purine or pyrimidine base or abasic nucleotides. In the context of the present invention, the “oligonucleotide” includes not only those with conventional bases, sugar residues and internucleotide linkages, but also those that contain modifications of any or all of these three moieties.

As used herein, the terms “nucleic acid” “polynucleotide” and “oligonucleotide” are used interchangeable herein and refer to a deoxyribonucleotide or ribonucleotide polymer in either single- or double-stranded form, and unless otherwise limited, encompasses known analogs of natural nucleotides that hybridize to nucleic acids in a manner similar to naturally-occurring nucleotides. Examples of such analogs include, without limitation, phosphorothioates, phosphoramidates, methyl phosphonates, chiral-methyl phosphonates, 2-O-methyl ribonucleotides, and peptide-nucleic acids (PNAs).

Sample: As used herein, the term “sample” refers to any composition that might contain a target of interest to be analyzed including, but not limited to, biological samples obtained from subjects (including humans and animals as detailed below), samples obtained from the environment for example soil samples, water samples, agriculture samples (including plant and crop samples), or food samples. Food samples may be obtained from fresh food, processed/cooked food or frozen food.

Sensitivity: As used herein, the term “sensitivity” means the ability of a detection molecule to bind to a target molecule.

Specifically binds: as used herein, the term “specifically binds” means that an aptamer reacts or associates more frequently, more rapidly, with greater duration and with greater affinity with a particular target molecule, than it does with alternative target molecules. For example, an aptamer that specifically binds to a target allergen binds that allergen or a structural part or fragment thereof with greater affinity, avidity, more readily, and/or with greater duration than it binds to unrelated allergen protein and/or parts or fragments thereof. It is also understood by reading this definition that, for example, an aptamer that specifically binds to a first target may or may not specifically bind to a second target. As such. “specific binding” does not necessarily require exclusive binding or non-detectable binding of another molecule, this is encompassed by the term “selective binding”. The specificity of binding is defined in terms of the comparative dissociation constants (Kd) of the aptamer for target as compared to the dissociation constant with respect to the aptamer and other materials in the environment or unrelated molecules in general. Typically, the Kd for the aptamer with respect to the target will be 2-fold, 5-fold, or 10-fold less than the Kd with respect to the target and the unrelated molecule or accompanying molecule in the environment. Even more preferably, the Kd will be 50-fold, 100-fold or 200-fold less.

Target: as used herein, the term “target” and “target molecule” refers to a molecule which may be found in a tested sample and which is capable of binding to a detection molecule such as an aptamer or an antibody.

EQUIVALENTS AND SCOPE

Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments in accordance with the invention described herein. The scope of the present invention is not intended to be limited to the above Description, but rather is as set forth in the appended claims.

In the claims, articles such as “a,” “an,” and “the” may mean one or more than one unless indicated to the contrary or otherwise evident from the context. Claims or descriptions that include “or” between one or more members of a group are considered satisfied if one, more than one, or all of the group members are present in, employed in, or otherwise relevant to a given product or process unless indicated to the contrary or otherwise evident from the context. The invention includes embodiments in which exactly one member of the group is present in, employed in, or otherwise relevant to a given product or process. The invention includes embodiments in which more than one, or the entire group members are present in, employed in, or otherwise relevant to a given product or process.

It is also noted that the term “comprising” is intended to be open and permits but does not require the inclusion of additional elements or steps. When the term “comprising” is used herein, the term “consisting of” is thus also encompassed and disclosed.

Where ranges are given, endpoints are included. Furthermore, it is to be understood that unless otherwise indicated or otherwise evident from the context and understanding of one of ordinary skill in the art, values that are expressed as ranges can assume any specific value or subrange within the stated ranges in different embodiments of the invention, to the tenth of the unit of the lower limit of the range, unless the context clearly dictates otherwise.

In addition, it is to be understood that any particular embodiment of the present invention that falls within the prior art may be explicitly excluded from any one or more of the claims. Since such embodiments are deemed to be known to one of ordinary skill in the art, they may be excluded even if the exclusion is not set forth explicitly herein. Any particular embodiment of the compositions of the invention (e.g., any antibiotic, therapeutic or active ingredient; any method of production, any method of use; etc.) can be excluded from any one or more claims, for any reason, whether or not related to the existence of prior art.

It is to be understood that the words which have been used are words of description rather than limitation, and that changes may be made within the purview of the appended claims without departing from the true scope and spirit of the invention in its broader aspects.

While the present invention has been described at some length and with some particularity with respect to the several described embodiments, it is not intended that it should be limited to any such particulars or embodiments or any particular embodiment, but it is to be construed with references to the appended claims so as to provide the broadest possible interpretation of such claims in view of the prior art and, therefore, to effectively encompass the intended scope of the invention.

EXAMPLES Example 1: Conjugating Aptamers (Specific to Peanut Allergen Ara H1) to Magnetic Beads

An aptamer against the Ara h 1 allergen protein which is described by Tran et al. in Selection of aptamers against Ara h 1 protein for FO-SPR biosensing of peanut allergens in food matrices. Biosensors and Bioelectronics, 2013, 43, 245-251 (incorporated herein by reference in its entirety), was used to design a signaling polynucleotide and conjugated to magnetic beads. The sequence of this aptamer is shown below (SEQ ID NO: 96).

5′TCGCACATTCCGCTTCTACCGGGGGTCGAGCTGAGTGGATGCGAA TCTGTGGGTGGGCCGTAAGTCCGTGTGTGCGAA3′ (SEQ ID NO.: 96)

A short nucleic acid sequence containing 5 nucleotide residues was designed to be complementary to the 3′-end residues of the T-modified aptamer of SEQ ID NO: 96. Alternatively, the sequence may be complementary to the 5′-end residues of the T-modified aptamer of SEQ ID NO: 96. One end of the complementary sequence was labeled with a fluorophore, Texas Red.

Three reactions were used to conjugate the aptamer to magnetic beads. The sequence was modified with a thiol (—SH) modifier at either the 5′end or 3′end (FIG. 1A and FIG. 1B). Magnetic beads were then linked to the 5′end (as shown in FIG. 1A) or to the 3′end (as shown in FIG. 1B) of the aptamer through covalent bonds. In particular, the thiol-modified aptamer, including 5′thiol and 3′thiol, was linked to magnetic beads by maleimide linkage. The Texas Red labeled complementary sequence was annealed to form a double stranded hybrid at the other end of the aptamer conjugated to magnetic beads, generating a magnetic bead conjugated signaling polynucleotide (SPN) (See FIG. 1A and FIG. 1B).

Alternatively, the aptamer was modified with a primary amine group at the 5′end or 3′end. The amine modified aptamer was attached to magnetic beads via carbodiimide chemical reaction. Magnetic carboxylated speedbeads were used (GE Healthcare Life Science, Cat. Log No.: XX). The Texas Red labeled complementary sequence was annealed to the aptamer at the 3′end, forming a magnetic bead conjugated signaling polynucleotide (SPN) (shown in FIG. 1C). Alternatively, the 5-nt complementary sequence was labeled with either Cy5 or Alex647 at one end (5′end or 3′end).

Amine Reaction

Amine-modified DNA molecules at either 5′ end of 3′ end were coupled to magnetic carboxylated speedbeads (GE Healthcare, USA) through carbodiimide chemical reaction. Carboxyl modified beads were first incubated with EDC/NHS (N-hydroxysuccinimide) prior to the addition of amine-modified DNA molecules. After EDC/NHS reaction, the carboxyl groups (—COOH) were activated for direct reaction with primary amines via amide bond formation. Amine-modified DNA molecules were mixed with the beads and the coupling reaction of beads and DNA occurred in water. After the reaction, a TRIS buffer was used to block/occupy the unreacted sites.

Thiol Reaction

Thiol-modified DNA molecules at either 5′ end of 3′ end were coupled to magnetic carboxylated speedbeads (GE Healthcare. USA) through amino-polyethylene-glycol maleimide linkage (2HN-PEG-Maleimide). The carboxyl groups (—COOH) on the surface of beads were activated first using water soluble EDC (1-ethyl-3-(˜3-dimethylaminopropyl) carbodiimide hydrochloride) and then by 2-HN-methoxypolyethylene glycol (PEG). The beads were incubated with EDC and PEGs in MES (4-morpholinoethanesulfonic acid) reaction buffer for 2 hours (30 min×4 sonicator bath). Activated beads were then mixed with thiol-modified DNA molecules and incubated with DTT (Dithiothreitol) in water.

Example 2: Reading of Fluorescence Signaling for Magnetic Beads Conjugated SPN in Detection of a Target Molecule

The study tested an experimental procedure for obtaining fluorescence readings and thereby determining the effectiveness of signaling polynucleotides in identifying and quantifying a molecular target such as an allergen protein in a food sample.

Peanut was diluted to an appropriate concentration in double-distilled water, ranging from 0 ppm to 500 ppm. SPN-magnetic bead conjugates as described in Example 1 were diluted in solution/buffer either HEPES/Tween, PBS/BSA or T-buffer (Tris pH8 100 mM NaCl, 50 mM KCl, 10 mM MgCl 0.5% Sodium Deoxcholate 0.1% Gelatin 1% Triton 0.1% SDS) at various concentrations. Peanut samples and SPN-magnetic bead conjugates were mixed and incubated for a period of time. The fluorescent signals before and after the reaction were detected and measured. In one study in which magnetic beads and SPN-complement were configured as illustrated in FIG. 1A, the fluorescent signals from Texas Red dye was decreased after the allergen binding (shown in FIGS. 2A to 2C). The relative fluorescent unit (RFU) indicates that Texas Red signal is dropped off after the peanut allergen target binds the SPN in a concentration dependent manner. It also shows that the complementary sequence could affect the signal decrease. As seen in FIGS. 2A and 2B, the complementary sequence could affect the signaling quencher after the binding of the target allergen. The sequence comprising 5 complementary nucleotides and 5nt polyA displayed a significantly fluorescence off (92% decrease) (C3 in FIG. 2B), while the sequence comprising 15 (C1 in FIG. 2A) or 10 (C2 in FIG. 2A) complementary nucleotides displays a moderate signal decrease.

Food samples spiked with peanut including Poptart, Graham crackers, Oreo, Blue Frosting were tested for signal decrease using 5′thiol modified SPN conjugated magnetic beads. As illustrated in FIG. 3 and FIG. 4, 5′ thiol modification displays significant fluorescent signal decrease in all foods tested and at different concentrations of target allergen, peanut (FIG. 3).

Comparison of signal detection using magnetic beads conjugated with 5′thiol modified SPNs and magnetic beads conjugated with polyA3′thiol modified SPNs suggest that 5′thiol modification displays more significant decrease than polyA3′thiol modification (See Table 6). About 40% of signal decrease was detected with magnetic beads conjugated with 5′thiol modified SPNs, while only about 20% of signal decrease was detected with magnetic beads conjugated with polyA3′thiol modified SPNs. The fluorescent measure also indicates that thiol modification displays more significant decrease than amine modification (data not shown).

TABLE 6 Fluorescent signal measure (RFU) (5′thiol v. 3′polyA thiol) Peanut (ppm) 0.0 0.5 5 50 500 Magnetic beads with 5′thiol modified aptamers 100 nM 19394.5 12896.9 9233.6 9376.4 8885.3  1 μM 34037.8 33582.8 32449.6 31283.4 30118.7  2.5 μM 36535.8 34252.9 33767.1 33926.5 32535 Magnetic beads with PolyA 3′thiol modified aptamers 100 nM 18888.4 15053.6 15249.9 15554.5 15387.1  1 μM 25213.2 25691.6 25303.1 24456.2 24404.7  2.5 μM 36515.3 34852.5 34342.5 32904 34064.1

Example 3: Amine-SPN Conjugates

As described in Example 1, amine-modified SPNs were annealed with the 5-nt complementary sequences (at a ratio of 1:5). The SPN-complement complex was conjugated to magnetic beads. The complementary sequence was labeled with Cy5 or Alex647, respectively. The SPN-magnetic bead conjugates were incubated with different concentrations of peanut flour (from 0 ppm to 500 ppm) at 37° C. Fluorescent signals were recorded after the incubation. As shown in Table 7, both dyes display significant signal decreases as peanut concentration increases, indicating more allergen proteins bind the SPN and detach the complementary sequences from the SPNs.

TABLE 7 Amine-SPN with peanut Peanut SPN 0 ppm 0.5 ppm 5 ppm 50 ppm 500 ppm Alex647 500 nM 9026 11617 11211 13074 10112  2.5 nM 22583 17662 21953 21380 18007 Cy5 500 nM 8102 6600 7762 9364 7431  5 nM 40595 39622 38021 32525 30101

Example 4: Thiol-SPN Conjugates

As described in Example 1, thiol-modified oligonucleotides were annealed with the 5-nt complementary sequences (at a ratio of 1:5). The SPN-complement complexes were conjugated to magnetic beads. The complementary sequence was labeled with Cy5 or Alex647, respectively. The SPN-magnetic bead conjugates were incubated with different concentrations of peanut flour (from 0 ppm to 500 ppm) at 37° C. Fluorescent signals were recorded after the incubation. As shown in Table 8, both dyes display significant signal decreases as peanut concentration increases, indicating more allergen proteins bind the SPN and detach the complementary sequences from the SPNs. As shown in Table 8, when the SPN is at high concentration, 1000 nM, Cy5 labeled signal decreases as the peanut concentration increases.

TABLE 8 Thiol-SPN with peanut Peanut SPN 0 ppm 0.5 ppm 5 ppm 50 ppm 500 ppm Alex647  500 nM 14806.8 15377.6 15231.7 14362.7 15001.6 1000 nM 35980.7 37720.1 36920 34901.3 36660.1 Cy5  500 nM 20692.3 20838.9 27197.2 28255.5 27519.7 1000 nM 28789.8 28290.8 20019.6 20162.1 19975

Example 5: Examining the Effect of Washing Step and Reaction Conditions on Signal Detection

Various parameters may affect the stability of nucleic acids immobilized on magnetic beads and their interaction with target allergens in a test sample. Tables 9 and 10 illustrate the fluorescent reading in various conditions tested. The data suggests that doubling Maleimide concentration enables signal decrease using a higher concentration of SPN. However the decrease doesn't retain more than 50% (Table 9). Shaking the SPN solution prior to the signal reading to re-suspend magnetic beads is critical for accurate signal measurement. It can cause about 65% decrease in signal (Table 10). The data also suggests that the step of washing beads after reaction, extraction buffer and annealing conditions affect the signal detection (Table 10).

TABLE 9 Fluorescent signal measure (RFU) (2XMaleimide/40 mg) Magnetic beads with 5′thiol modified aptamers Peanut (ppm) 0.0 5 50 500 100 nM 30786.4 15740.5 17604.1 17452.1 1 μM 27295.6 20574 15591.3 15271.4 5 μM 47497.8 43324.9 42758.1 38351.5

TABLE 10 Fluorescent signal measure (RFU) Magnetic beads with 5′thiol modified aptamers Peanut (ppm) 0.0 0.5 5 50 500 Extraction buffer; shaken 6152.8 4635 5170 5713 5304.5 before read PBS with BSA; shaken 30504.5 10861.3 7620.5 6253.7 7037 before read Exaction buffer; not 7051 5584.5 7660.8 6642.8 7567.3 shaken PBS with BSA; not 8966 7685.8 8983 7269 9062.3 shaken

Effect of Wash Components on Signal Detection

Reaction mixtures comprising polyA-thiol modified SPNs and peanuts were washed before signal detection using PBS buffer containing BSA (Bovine serum albumin). As compared with the signal after washing with PBS only, noticeable signal decrease is detected as peanut concentration is increased, indicating that BSA can facilitate removal of the complementary sequences after allergen binding (Table 11).

TABLE 11 BSA effect on signal detection Peanut diluted in PBS/BSA SPN 500 nM 2.5 nM 500 nM 2.5 nM peanut (Alex647) (Alex647) (Cy5) (Cy5)  0 ppm 16,692 18587 14458 33500  5 ppm 16832 18078 13304 34606 500 ppm 16731 17841 12874 37788 Peanut diluted in PBS only (no BSA) SPN 500 nM 2.5 nM 500 nM 2.5 nM (Alex647) (Alex647) (Cy5) (Cy5)  0 ppm 19953.9 21356.3 13589.4 39577.4  5 ppm 16865.6 19508 14558.3 41638.4 500 ppm 16135.1 17034 12959.4 33267.1

Washing Buffer Containing Detergent

SPN-complement complexes with Texas Red, complementary sequences labeled with Texas red, and fluorophore Texas Red alone were washed with PBS buffer containing Tween-20 at various concentrations. The fluorescent signals (RFU) after washing were detected and compared.

TABLE 12 signal (RFU) after PBS/Tween-20 washing Amine- Complement SPN/complement alone Texas red PBS only 13425.4 5554.9 1778.8 PBS plus 0.05% Tween 11249.8 5133.5 1581.3 PBS plus 0.1% Tween 5683 2342.9 903

Example 6: Ratio of Oligonucleotides and Complementary Sequences

As shown in Examples 3 and 4, the high ratio 1:5 of aptamer oligonucleotides and complementary sequences gives a high fluorescent signal. A ratio 1:2 of aptamer oligonucleotides and complementary sequences was tested for signal detection.

TABLE 13 SPN: complementary sequence at a ratio of 1:2 SPN Alex647 Cy5 100 nM 2167.5 1809.9 500 nM 14967 10499.3 1 μM 29429.2 23651.2 2.5 μM 30386.4 30418.5 5 μM 21663.9 39843.3

Magnetic beads conjugated with complexes of amine-SPN and its complementary sequences labeled with Cy5 in which the amine-SPN molecules and CY-5-labeled complementary sequences is at a ratio of 1:2, were incubated with peanut flour at concentrations from 0 to 500 ppm. Signals were detected and as shown in Table 14, signal decreases as peanut concentration increases.

TABLE 14 Signal detection with peanut flour Amine-SPN and complementary sequence labeled with Cy5 10 μl Magnetic 20 μl magnetic peanut bead conjugates bead conjugates 0 ppm 23703.4 38756.8 0.5 ppm 27125.8 38830 5 ppm 26329.7 38264.1 50 ppm 25576.2 36271 500 ppm 19263.4 33445.4 2500 ppm 8798.1 17685.8

Example 7: Magnetic Beads Absorbance

To test if the same amount of beads are analyzed during target detection, the absorbance signals were analyzed in parallel with the fluorescent signal. Magnetic beads conjugated with SPN-complement complexes of amine-SPN and its complementary sequence (5nt in length) labeled with Cy5 in which the amine-SPN molecules and CY-5-labeled complementary sequences is at a ratio of 1:2, were incubated with peanut flour at concentrations from 0 to 500 ppm. Absorbance by beads was measured. The absorbance data indicates a change in absorbance when magnetic beaded conjugated to SPNs are exposed to higher concentrations of peanut flour (See Table 15).

TABLE 15 Absorbance by beads with amine-SPNs Peanut Amine-SPN 0 ppm 0.5 ppm 5 ppm 50 ppm 500 ppm  50 nM 454.3 443.2 438.5 405.6 385.9 250 nM 13796.8 14562.2 15624.6 13546.4 10750.2 500 nM 30671.6 33112.6 33363.3 31182 25944.6

Similarly, magnetic beads conjugated with SPN-complement complexes of thiol-SPN and its complementary sequence (10 nt in length) labeled with Texas red in which the amine-SPN molecules and Texas red-labeled complementary sequences is at a ratio of 1:2, were incubated with peanut flour at concentrations from 0 to 500 ppm. Absorbance by beads was measured. As shown in Table 16, the absorption data indicates no changes in absorbance with beads conjugated to thiol-SPNs.

TABLE 16 Absorbance by beads with thioL-SPNs Peanut Thiol-SPN 0 ppm 0.5 ppm 5 ppm 50 ppm 500 ppm 250 nM 12357.8 12397.8 12087.6 11863.2 10599.2 500 nM 35442 36624 35181.6 36071.2 32547.8

Example 8: DNA Printing on the Surface of Glass Slides Optimize the Printing Protocol

3 complementary sequences ranging in length between 10-15 nucleotides with a 3′amine modification are used for the test. The DNA sequences are attached and printed on the surface of the glass slides using a variety of DNA loading densities and slide coatings.

Screen for Complementary Sequences for a Selected Aptamer

A microarray-based screen is used to select complementary DNA sequences that only bind the aptamer when it is not bound to the allergen protein. An aptamer (SEQ ID NO. 353 and SEQ ID NO. 307) specific to peanut allergen protein AraH1 and an aptamer (SEQ ID NO. 564) specific to nut were selected. About 40 short sequences that are complementary to different portions of each aptamer are designed based on the aptamer sequence (See Table 17). These sequences range in length between 10-20 nucleotides. The short sequences (also referred to as anchor or linker sequences) are printed on the surface of the glass slide using the printing protocol optimized previously.

TABLE 17 Short complementary sequences SEQ ID NO. Complement (5′-3′) SEQ ID NO. Complement (5′-3′) AraH1  96 TCGCACATTCCGCTTCTACC P10 307 TAGGGAAGAGAAGGACATATG GGGGGGGTCGAGCTGAGTGG ATGTCAGTCGATGGATGTGGT ATGCGAATCTGTGGGTGGGC TGTGCTCGTCTTGACTAGTAC CGTAAGTCCGTGTGTGCGAA ATGACCACTT A_1 697 TTCGCACACA P_1 739 AAGTGGTCAT A_2 698 ACACACGGAC P_2 740 GTCATGTACT A_3 699 CGGACTTACG P_3 741 GTACTAGTCA A_4 700 TTACGGCCCA P_4 742 AGTCAAGACG A_5 701 GCCCACCCAC P_5 743 AGACGAGCAC A_6 702 CCCACAGATT P_6 744 AGCACAACCC A_7 703 AGATTCGCAT P_7 745 AACCCACATC A_8 704 CGCATCCACT P_8 746 ACATCCATCG A_9 705 CCACTCAGCT P_9 747 CATCGACTGA A_10 706 CAGCTCGACC P_10 748 ACTGACATCA A_11 707 CGACCCCCCC P_11 749 CATCATATGT A_12 708 CCCCCGGTAG P_12 750 TATGTCCTTC A_13 709 GGTAGAAGCG P_13 751 CCTTCTCTTC A_14 710 AAGCGGAATG P_14 752 TCTTCCCTA A_15 711 GAATGTGCGA P_15 753 AAGTGGTCATGTACT A_16 712 TTCGCACACACGGAC P_16 754 GTCATGTACTAGTCA A_17 713 ACACACGGACTTACG P_17 755 GTACTAGTCAAGACG A_18 714 CGGACTTACGGCCCA P_18 756 AGTCAAGACGAGCAC A_19 715 TTACGGCCCACCCAC P_19 757 AGACGAGCACAACCC A_20 716 GCCCACCCACAGATT P_20 758 AGCACAACCCACATC A_21 717 CCCACAGATTCGCAT P_21 759 AACCCACATCCATCG A_22 718 AGATTCGCATCCAT P_22 760 ACATCCATCGACTGA A_23 719 CGCATCCACTCAGCT P_23 761 CATCGACTGACATCA A_24 720 CCACTCAGCTCGACC P_24 762 ACTGACATCATATGT A_25 721 CAGCTCGACCCCCCC P_25 763 CATCATATGTCCTTC A_26 722 CGACCCCCCCGGTAG P_26 764 TATGTCCTTCTCTTC A_27 723 CCCCCGGTAGAAGCG P_27 765 CCTTCTCTTCCCTA A_28 724 GGTAGAAGCGGAATG P_28 766 AAGTGGTCATGTACTAGTCA A_29 725 AAGCGGAATGTGCGA P_29 767 GTCATGTACTAGTCAAGACG A_30 726 TTCGC ACACACGGACTTACG P_30 768 GTACTAGTCAAGACGAGAC A_31 727 ACACACGGACTTACGGCCCA P_31 769 AGTCAAGACGAGCACAACCC A_32 728 CGGACTTACGGCCCACCCAC P_32 770 AGACGAGCACAACCCACATC A_33 729 TTACGGCCCACCCACAGATT P_33 771 AGCACAACCCACATCCATCG A_34 730 GCCCACCCACAGATTCGCAT P_34 772 AACCCACATCCATCGACTGA A_35 731 CCCACAGATTCGCATCCACT P_35 773 ACATCCATCGACTGACATCA A_36 732 AGATTCGCATCCACTCAGCT P_36 774 CATCGACTGACATCATATGT A_37 733 CGCATCCACTCAGCTCGACC P_37 775 ACTGACATCATATGTCCTTC A_38 734 CCACTCAGCTCGACCCCCCC P_38 776 CATCATATGTCCTTC TCTTC A_39 735 CAGCTCGACCCCCCCGGTAG P_39 777 TATGTCCTTCTCTTCCCTA A_40 736 CGACCCCCCCGGTAGAAGCG P_40 A_41 737 CCCCCGGTAGAAGCGGAATG P_41 A_42 738 GGTAGAAGCGGAATGTGCGA P_42

Each of 16-array slides is coated with 3 copies of the 50 sequences, giving a total of 150 sequences per array (see chip layout in Table 18) using the printing protocol optimized previously. The binding of the short sequences to its target aptamer is tested using either an attachment or detachment protocol detailed below. The aptamer is labeled on the 5′ end with a fluorescent dye Cy5 which is used to quantify the aptamer bound to the plate. The allergenic protein is prepared into a serial dilution of five different concentrations (e.g., 0 ppm, 1 ppm, 10 ppm, 100 ppm, and 1000 ppm). The output of the experiment is relative Cy5 reads from the protein curve as well as the negative controls. Table 17 shows an example of the screen chip layout. The screen consists of three 16-array slides. Each array is designed to have 3 copies of the 50 sequences (150 samples total). For each experimental slide, a 5-point protein curve (×3) and a buffer control are included (a full 16 array slide).

TABLE 18 Screen chip layout Slide Treat- No. ment Slide setup 1 Attach- 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm ment 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm protocol 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm buffer (tripli - cates) 2 Detach- 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm ment 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm protocol 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm buffer (tripli- cates) 3 Controls 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm (dupli- 0 ppm 1 ppm 10 ppm 100 ppm 1000 ppm cates) buffer buffer aptamer aptamer aptamer aptamer

Attachment Assay

For the attachment protocol, a fixed concentration of aptamer is mixed with increasing concentrations of the allergen protein for 1 min to allow the aptamer to bind to the allergen protein. The protein-aptamer mixture is then added to the wells of the plate and incubated for 1 min at room temperature, washed, and measured for fluorescence. The controls for the experiment include determining fluorescence of the microarray wells with either only the aptamer or protein not previously incubated with the aptamer, as well as fluorescence with only the short sequences present. Aptamer that is protein-free attaches to the short sequences immobilized on the plate and contributes to the fluorescence reading. Protein-bound aptamer does not attach to the plate and is washed away. If the short immobilized DNA sequence only binds the protein-free aptamer, decreasing fluorescence signal is observed with an increasing concentration of the protein, as the higher the protein concentration the less protein-free aptamer is available to bind to the short sequence on the microarray. If the short sequence cannot differentiate between protein-bound and unbound aptamer, a similar fluorescence intensity is observed regardless of the concentration of the protein.

Detachment Assay

For the detachment protocol, the aptamer is added to the wells of the plate and incubated for 1 min at room temperature, washed, and measured for fluorescence. Protein is added to the plate at five different concentrations, incubated for 1 min, washed, and measured for fluorescence again. The controls of the experiment are the same as described for the attachment protocol. If the short sequence only binds the protein-free aptamer, a drop in fluorescence signal is observed when protein is added. The magnitude of the drop increases with an increasing concentration of the protein, as the higher the protein concentration the more aptamers detach from the short immobilized sequence. If the short sequence cannot differentiate between protein-bound and unbound aptamer, a similar fluorescence intensity is observed regardless of the concentration of the protein.

The top 3 short sequences are selected based on the screen results and validated using a second microarray. Each one of the 3 sequences is printed in 50 spots per array, giving a total of 150 sequences. The binding to the short sequences is tested using either an attachment or detachment protocol as described above. The validation assay incorporates control proteins and control test matrices (see chip layout in Table 18). Relative Cy5 reads from different protein concentrations as well as the negative controls are compared. The best candidate meets the following criteria: (a) specific binding to the corresponding aptamer, (b) easy detachment from the bound aptamer in the presence of the allergenic protein, and (c) minimal background/non-specific binding. The selected complementary sequence is used to form SPN-complement complexes.

Table 19 shows the chip layout for the validation assay. A set of 12, 16-array slides are used for the attachment assay and another 12 are used for the detachment assay. For each slide, a 5-point curve (×3) and a control are included (a full 16 array slide). Each spot of the 16 array slides contains 50 copies of the 3 candidates selected from the screen (150 samples total).

TABLE 19 Validation Chip layout Slide No. Category Slide setup 1 Test protein curve + aptamer in buffer 2 Test protein curve + aptamer in food 1 3 Test protein curve + aptamer in food 2 4 Test protein curve + aptamer in food 3 5 Control control protein + aptamer curve 1 6 Control control protein + aptamer curve 2 7 Control control protein + aptamer curve 3 8 Control aptamer, no protein 9 Control no aptamer in buffer 10 Control no aptamer in food 1 11 Control no aptamer in food 2 12 Control no aptamer in food 3

Example 9: Validation of Detection Sensitivity of SPN-Magnetic Beads Conjugates

As discussed in Example 1, 5′ Thiol modified short complementary sequences were conjugated to magnetic beads and aptamer specific to peanut allergen (SEQ ID NO. 96: 5′ (Texas Red) TCGCACATTCCGCTTCTACCGGGGGGTCGAGCTGAGTGGATGCGAATCTGTGGG TGGGCCGTAAGTCCGTGTGTGCGAA3′) was hybrided with the short linker nucleic acid molecules. The aptamer was labeled with Texas red at the 5′ end. The short linker sequence is AAAAATCAAGTGGTC with 5′ Thiol modification (SEQ ID NO. 778)

The SPN-magnetic bead conjugates were used as detection agents to validate the detection sensitivity in detection assays. Peanut was diluted in either buffer or cookie at 0 ppm, 5 ppm, 50 ppm and 500 ppm, respectively. The prepared peanut samples were reacted with SPN-magnetic bead conjugates (loaded in 96-well microplate) and signals were read using lab-grade LED based reader after incubation and wash. Under bench-top reaction conditions, peanut present either in buffer or in cookie can be detected at a low ppm using SPN-magnetic bead conjugates. The recorded signal indicates that the fluorescent signal is correlatively reduced when the concentration of peanut increases. At the concentration of 50 ppm (peanut commodity), a significant fluorescent signal reduction is recorded in buffer (FIG. 7A) and cookie (FIG. 7B). This observation confirms the 50 ppm detection sensitivity as shown in previous assays. In a similar assay, when peanut was added to other food samples, a significant signal reduction is seen at 50 ppm peanut (FIG. 8B). Comparison of food samples with peanut and those containing no peanut, at least 25% of signal reduction is observed in all samples compared (FIG. 8A). Food samples were chose based on their general concerns with allergic concerns. For example, cookie, cereal, chocolate and ice cream are commonly consumed; Blue frosting is high food coloring; Pizza is highly processed food which is hard to detect the presence of allergens using available detection assays such as the ELISA assay; and Ranch dressing is high in fat. This selection covers a broad range of matrices. These observations suggest that assays using SPN-magnetic bead conjugates can achieve a 50 ppm sensitivity with all food matrices being tested.

In order to further confirm the sensitivity of the SPN-magnetic bead conjugates based assay, over 20 different food matrices were spiked with peanut and tested for signal detection and its sensitivity. The 50 ppm sensitivity was confirmed on representative foods from each category as shown in Table 20.

TABLE 20 The detection sensitivity of SPN-magnetic bead conjugates Fluorescent signal reduction Food category Food 0 ppm peanut 50 ppm peanut Baked goods cookie 100% 71% Red Velvet Cake 100% 86% Oatmeal Cookie 100% 68% Waffer 100% 47% Sauses, dressings Dressing 100% 67% and Marinades salsa 100% 61% Tomato sauce 100% 81% Hummus 100% 77% Entrees Oatmeal 100% 73% Sausage 100% 67% Bread 100% 82% French Fries 100% 37% Pizza 100% 76% Chicken 100% 60% Desserts Vanilia Pudding 100% 68% Vanilla Oreo 100% 79% Meringue 100% 64% Blue Frosting 100% 64% Sorbet 100% 21% Ice Cream 100% 79% Blueberry Yogurt 100% 82% Grape Jelly 100% 41%

The detection sensitivity of SPN-magnetic bead conjugates was further confirmed using different fluorescent signal readers. The signal reading was recorded and analyzed using a lab-grade LED based reader as well as a designed optical sensor. When the detection assay was carried out using Data shown in Table 21 indicate that the detection sensitivity is not affected when using different signal readers. The designed optical sensor is comparable to the laboratory-standard microplate reader (e.g., FIGS. 8A and 8B; and Table 20) and can differentiate between 0 ppm and 50 ppm peanut in food with 95% confidence.

TABLE 21 The detection sensitivity of SPN-magnetic bead conjugates Fluorescent signal reduction Food 0 ppm peanut 50 ppm peanut Cookie 100% 62% Sorbert 100% 28% Frosting 100% 72% Dressing 100% 67% Pizza 100% 72% Cracker 100% 53% Cookie 100% 65% Ice cream 100% 65% Biscuit 100% 62% Pretzel 100% 57% Waffer 100% 47% Poptart 100% 45%

Example 10: Detection Assays with Nucleic Acid Coated Chips

Chips were coated with short complementary DNA sequences that bind the aptamer only when it is not bound to the allergen protein. These short nucleic acid anchor sequences specific to the aptamers (SEQ ID NO. 307, SEQ ID NO. 404 and SEQ ID NO. 304) which bind to peanut allergen protein were used to coat the glass. These anchor sequences are about 10 nt in length. The short anchor sequences are further modified to contain 5 (polyA) at one end to pull the sequence away from the surface. A 6 carbon or 12 Carbon linker is further added to the sequences to pull them further away from the surface. An amine attachment is added to print the sequences to the surface of the chip. The sequences and modification of the anchor/linker DNA molecules are listed in Table 22. Prepared peanut containing samples were incubated with a fixed concentration of SPNs specific to the peanut allergen and filtered to remove unbound food particles. The aptamers were labeled with Cy5 at the 5′ end. The mixture was incubated with the chip coated with short linker/anchor sequences. After incubation and wash, the fluorescent reading was recorded using a lab grade LED based reader, as well as the designed optical sensor. The anchor sequences that generate the most specific and sensitive signals are selected for further validation.

TABLE 22 Sequences used to coat the solid surface (chip) and their modifications Name Sequence Modification SEQ ID NO. AP_1 /5AmMC6/TTCGCACACA 5′ 6CAmine 697 AP_2 /5AmMC6/ACACACGGAC 5′ 6CAmine 698 AP_3 /5AmMC6/CGGACTTACG 5′ 6CAmine 699 AP_4 /5AmMC6/TTACGGCCCA 5′ 6CAmine 700 AP_5 /5AmMC6/GCCCACCCAC 5′ 6CAmine 701 AP_6 /5AmMC6/CCCACAGATT 5′ 6CAmine 702 AP_7 /5AmMC6/AGATTCGCAT 5′ 6CAmine 703 AP_8 /5AmMC6/CGCATCCACT 5′ 6CAmine 733 AP_9 /5AmMC6/CCACTCAGCT 5′ 6CAmine 705 AP_10 /5AmMC6/CAGCTCGACC 5′ 6CAmine 706 AP_11 /5AmMC6/CGACCCCCCC 5′ 6CAmine 707 AP_12 /5AmMC6/CCCCCGGTAG 5′ 6CAmine 708 AP_13 /5AmMC6/GGTAGAAGCG 5′ 6CAmine 709 AP_14 /5AmMC6/AAGCGGAATG 5′ 6CAmine 710 AP_15 /5AmMC6/GAATGTGCGA 5′ 6CAmine 711 3_1 /5AmMC6/aaaaaTCAAGTGGTC 5′ 6CAmine 778 3_2 /5AmMC6/aaaaaTGGTCATGTA 5′ 6CAmine 779 3_3 /5AmMC6/aaaaaTGTACTAGT 5′ 6CAmine 780 3_4 /5AmMC6/aaaaaTACTAGTCAA 5′ 6CAmine 781 5_1 /5AmMC6/aaaaaATCAT ATGTC 5′ 6CAmine 782 5_2 /5AmMC6/aaaaaATGTCCTTCT 5′ 6CAmine 783 5_3 /5AmMC6/aaaaaCTTCTCTTCC 5′ 6CAmine 784 5_4 /5AmMC6/aaaaaCTCTTCCCTA 5′ 6CAmine 785 P1_10 /5AmMC6/aaaaaCATCGACTGACA 5′ 6CAmine 786 P2_8 /5AmMC6/aaaaaCCATCGATGC 5′ 6CAmine 787 P2_18 /5AmMC6/aaaaaCTACACCCACATC 5′ 6CAmine 788 AP_1_PA /5AmMC6/aaaaaTTCGCACACA 5′ 6CAmine 789 AP_2_PA /5AmMC6/aaaaaACACACGGAC 5′ 6CAmine 790 AP_3_PA /5AmMC6/aaaaaCGGACTTACG 5′ 6CAmine 791 AP_4_PA /5AmMC6/aaaaaTTACGGCCCA 5′ 6CAmine 792 AP_5_PA /5AmMC6/aaaaaGCCCACCCAC 5′ 6CAmine 793 AP_6_PA /5AmMC6/aaaaaCCCACAGATT 5′ 6CAmine 794 AP_7_PA /5AmMC6/aaaaaAGATTCGCAT 5′ 6CAmine 795 AP_8_PA /5AmMC6/aaaaaCGCATCCACT 5′ 6CAmine 796 AP_9_PA /5AmMC6/aaaaaCCACTCAGCT 5′ 6CAmine 797 AP_10_PA /5AmMC6/aaaaaCAGCTCGACC 5′ 6CAmine 798 AP_11_PA /5AmMC6/aaaaaCGACCCCCCC 5′ 6CAmine 799 AP_12_PA /5AmMC6/aaaaaCCCCCGGTAG 5′ 6CAmine 800 AP_13_PA /5AmMC6/aaaaaGGTAGAAGCG 5′ 6CAmine 801 AP_14_PA /5AmMC6/aaaaaAAGCGGAATG 5′ 6CAmine 802 AP_15_PA /5AmMC6/aaaaaGAATGTGCGA 5′ 6CAmine 803

Example 11: Sensitivity of the Detection Assay Based on Nucleic Acid Coated Chip

Peanut detection using nucleic acid coated chips was evaluated in different detection assays and with different food matrices. The sensitivity of the detection assay based on nucleic acid coated chips was validated and confirmed. In this study, the anchor/linker sequence (5′ 12C-Amine) AAAAATTCGCACACA (SEQ ID NO. 789) was printed on the surface of the chip. As shown in FIG. 9A, peanut diluted in buffer at various concentrations was incubated with peanut specific SPN (SEQ ID NO. 96: 5′ (Cy5) TCGCACATTCCGCTTCTACCGGGGGGGTCGAGCTGAGTGGATGCGAATCTGTGGG TGGGCCGTAAGTCCGTGTGTGCGAA3′) and run through the DNA coated solid surface of the chip, the fluorescent signal recorded in nucleic acid coated chip based detection assay is correlated with the increased peanut concentration in buffer. The signal change can be detected as a low concentration of peanut (e.g., 5 ppm). Similarly, peanut diluted spiked in shortbread at various concentrations was incubated with peanut specific SPN and run through the DNA coated solid surface of the chip, the fluorescent signal recorded in nucleic acid coated chip based detection assay is correlated with the increased peanut concentration in buffer (FIG. 9A). The data also indicate that the SPN detection sensitivity is food dependent. In food matrices, the sensitivity is decreased as compared in simple buffer samples (FIGS. 9A and 9B).

Detection assays with nucleic acid coated chip were tested both on a designed reaction system (e.g., the rig), and the benchtop reaction and LED read. More than 20 food samples were tested and the detection sensitivity of the SPN in solid surface based assay is repeatable using different solid surfaces (see, e.g., FIGS. 10A and 10B). The designed reaction system contains a test cartridge the hold the extraction buffer and wash buffer (e.g., HEPES buffer and TGK T-Buffer). SPN molecules at various concentrations (5 nM, 10 nM, or 50 nM) are pre-loaded in the extraction buffer. The wash buffer does not have the SPN. The cartridge also holds the DNA coated chip inside a reaction chamber within the cartridge. A driving system is also provided to activate the cartridge, driving the homogenization of the food and controlling the flow of the sample during the reaction. It also has an optical system attached to measure the detection system. In both reaction settings, a comparable detection sensitivity can be achieved (FIGS. 10A and 10B). The same sensitivity of 12.5 ppm peanut protein (equal to 50 ppm peanut commodity) is also retained in diverse chocolate matrices as tested on the rig with nucleic acid coated chips (FIG. 10C).

Example 12. Comparison of Detection Sensitivity Between SPN-Magnetic Bead Conjugates and Nucleic Acid Coated Solid Surface (Chip)

Detection assays using SPN-magnetic bead conjugates and nucleic acid coated chips were validated in various conditions using a variety of different food samples. The detection sensitivity is confirmed in different conditions. For assays using SPN-magnetic bead conjugates, food samples without or with 50 ppm peanut were prepared using GentleMACS homogenizer and centrifuged. The processed samples were then incubated with SPN-magnetic bead conjugates and fluorescent signals were recorded using lab-grade LED based reader. The 50 ppm sensitivity was confirmed in 20 food samples tested (FIG. 11A). In a parallel study, food samples without or with 50 ppm peanut were prepared using rotor-dependent homogenizer and homogenized samples were filtered using 0.2 mm PES filter. The processed samples were then incubated with SPN-magnetic bead conjugates and fluorescent signals were recorded using lab-grade LED based reader. The 50 ppm sensitivity was confirmed in 5 food samples tested (FIG. 11C).

Detection assays were also performed using nucleic acid coated chips as described in Example 10. Food samples without or with 50 ppm peanut were prepared using GentleMACS homogenizer and centrifuged, or alternatively prepared using rotor-dependent homogenizer and filtered using 0.1 mm PES filter. The processed samples were then incubated with a fixed concentration of aptamer specific to peanut allergen. The mixed samples were added to the nucleic acid coated chips. After incubation and wash, the fluorescent signals were recorded using designed optical sensors. The 50 ppm sensitivity was achieved in different food samples (FIG. 11B) and was further confirmed in 9 food samples tested (FIG. 11D).

The sensitivity of SPN-magnetic beads and nucleic acid coated chips was also tested in different reaction settings such as standard bench-top reaction chamber and a designed reaction chamber (e.g., the rig). The rig is a benchtop fixture that includes a motor, syringe pump and valving the enables the homogenization of the food sample, filtering through a filter bed and running the sample over the reaction chamber in which the DNA coated chip is located. The rig enables controlled washing. The detailed conditions are listed in Table 23. In all conditions tested, the 50 ppm sensitivity can be achieved.

TABLE 23 Validation of assay sensitivity Fluorescent signal reduction 0 ppm 50 ppm Assay Assay conditions Food peanut peanut Magnetic GentleMACS homogenizer Lemon 100% 22% beads and centrifugation; Lab- sobert (N = 3) standard bench-top Shortbread 100% 67% reaction; designed optical cooike sensor Blue 100% 79% frosting Pizza 100% 70% Dressing 100% 84% Nucleic Designed Rotor- Lemon 100% 76% acid solid homogenizer and 1 mm sobert surface PES filter; Lab-standard Shortbread 100% 69% (N = 4) bench-top reaction; cooike designed optical sensor Blue 100% 67% frosting Pizza 100% 76% Dressing 100% 73% Magnetic Designed Rotor- Lemon 100% 36% beads homogenizer and bulk sobert (N = 2) filters; designed rig Shortbread 100% 65% reaction chamber; designed cooike optical sensor Blue 100% 72% frosting Pizza 100% 51% Dressing 100%  0% Nucleic Designed Rotor- Lemon 100% 36% acid solid homogenizer and 1 mm sobert surface PES filter; designed rig Shortbread 100% 50% (N = 3) reaction chamber; designed cooike optical sensor Blue 100% 72% frosting Pizza 100% 56% Dressing 100% 53%

Example 13: Optimizing Detection Assays on Solid Surface Limited Reaction Buffer

The detection assay run on nucleic acid coated solid surface (e.g., chip) was optimized in several aspects and its sensitivity was validated in various reaction conditions. The effect of buffer volume on the detection sensitivity was tested in one study. In the nucleic acid chip assay, when the reaction volume is decreased by 50% (2.5 ml) and only half of the sample size (0.25 g per sample) was used, the detection result indicates that limited buffer volume and reduced sample size has minimal effect on the detection sensitivity of SPNs and solid surface assays (FIG. 12).

Internal Control

To reduce background recording and signals from non-specific bindings, control signals to subtract these non-specific readings are important to optimize the assay. An internal control signal was recorded to correct signal measurement. The two control panels as shown in FIG. 13A contain the sequence GAAAAGTGCTCATCTGTGAACTCTAT (SEQ ID NO. 804) that has CY5 bound to on end and amine on the other side. The sequences are printed on the surface of the chip at various patterns (not shown) but keep the similar relevant positions to the detection area where DNA anchor/linker sequences specific to SPNs are printed (as the diagram shown in FIG. 13A). In general, control areas are located at various locations outside of the detection area on the chip. After sample incubation and wash, fluorescence signals from the detection area and control areas are read and analysed to indicate the concentration of allergen detected in the sample.

Concentration of MgCl2

Fluorescent signal is likely be affected by many factors such as salts and buffer concentration, etc. The concentration of MgCl2 in reaction buffer is to optimize the detection assay to achieve high-sensitive and intense signal. 0 mM to 120 mM MgCl2 was tested and MgCl2 was added either to extraction buffer or after food sample extraction and filtration. The results suggest that addition of MgCl2 to extraction buffer completely eliminates sensitivity. The MgCl2 concentration needs to be tightly controlled between 25 mM and 50 mM. Lower or higher concentration of MgCl2 affects both sensitivity and signal intensity (FIGS. 14A, 14B and 14C)

Optimization of Detection Assay on the Rig

In addition to internal control, various parameters that affect the efficiency of detection assay were optimized including the steps of pre-blocking the DNA coated chips, decreasing reaction time and washing. It is found that DNA-chip, the solid surface can be effectively blocked by BSA, which reduce non-specific signal. During the process of assaying, the reaction time can be decreased from 6 minutes to about 64 seconds. Optimized steps include removing air bubbles for both the reaction and wash, decreasing incubation time of food sample and SPNs, transitioning to a slow flow of incubation, increasing volume of reaction to flow over the chip and increasing flow rate of solution to accommodate the volume in 30 seconds. One example of the optimized reaction step and time is shown in Table 24.

TABLE 24 Optimization of reaction on the rig (solid surface) Step Time Sample Homogenization of food in 5 ml of buffer 40 Sec process with 20 nM SPN; Filtration 1 micron FES filter Reaction Prime Channels and remove BSA 4 Sec process Adding 500 ul of food and SPN filtrate 30 Sec Wash 500 ul 20 Sec Air dry 4 Sec Read 1 Sec

In this protocol of detection reaction within 64 seconds, the assay sensitivity is retained (FIG. 15).

Filtration

Different filters were tested and compared for efficiency in removing food particles and its effect on signal read. Three different filters: fish/netting, cotton/glass, and cotton/netting were tested and compared in 6 different food matrices spiked with peanut (Table 25). Dependent of food matrices, a different combination of filters may be used to increase allergen extraction from the sample; and to deplete other components such as fat and other particles.

TABLE 25 Filter comparison short- Ranch Bread Blue White Bagle- Dressing Cookie Frosting Frosting Bites (wishbone) Sorbert Cotton/glass 100% 100% 100% 100% 100% 100% 0 ppm peanut 100% 100% 100% 100% 100% 100% Cotton/glass  59%  77%  16%  63%  60%  85% 50 ppm  54%  59%  35%  67%  47%  51% peanut Fish/netting 100% 100% 100% 100% 100% 100% 0 ppm peanut 100% 100% 100% 100% 100% 100% Fish/netting /  76%  95%  72%  55%  85% 50 ppm  73%  54%  53%  83% /  75% peanut Cotton/netting 100% 100% / 100% 100%  0% 0 ppm peanut 100% 100% / 100% 100%  0% Cotton/netting  42%  49% /  9%  59%  0% 50 ppm  33%  60% /  79%  73%  0% peanut

Example 14: Stability of Detection Agents and Other Agents for Detection Assays

Components used for the present detection assay need to be stable at ambient temperature. Examples of agents and other parts employed to run an allergen assay, include extraction buffer, wash buffer, Flagged-SPN and DNA chips. The stability test indicates that fluorescent labeled SPN (e.g., Texas-Red labeled SPN) is stable and its activity remains at least for one month at various temperatures. (Table 26) as measured with fluorescent polarization (FP). After 9 month storage, significant fluorescent signal can still be detected (FIGS. 16A and 16B). Buffers used for the detection assay can remain stable for at least 9 month (FIGS. 16C and 16D).

TABLE 26 Stability of Texas-red labeled SPN activity at various temperatures Delta signal (mP) Day 0 Day 1 Day 2 Day 4 Week 2 Week 3 Week 4 4° C. 5000 152 153 143 153 154 148 128 500 114 109 108 105 106 92 75 50 36 27 22 37 31 24 21 5 4 7 (1) 8 6 8 8 25° C. 5000 152 151 148 149 164 158 141 500 114 99 98 107 115 104 81 50 36 26 20 35 35 27 21 5 4 2 2 12 4 6 4 42° C. 5000 152 147 136 152 161 190 160 500 114 104 119 109 119 121 103 50 36 22 31 33 34 34 26 5 4 1 4 10 5 3 3 

1.-56. (canceled)
 57. An allergen detection agent comprising: (a) a solid substrate; (b) an allergen binding signaling polynucleotide (SPN) comprising a nucleotide sequence that binds a target allergen and having a 3′ and 5′ end, and (c) a complement comprising a nucleotide sequence complementary to a region of the SPN sequence.
 58. The allergen detection agent of claim 57 further comprising a fluorophore.
 59. The allergen detection agent of claim 58 wherein the complement comprises 5-20 nucleotide residues, or 10-20 nucleotide residues.
 60. The allergen detection agent of claim 59 wherein the SPN is immobilized to the surface of the solid substrate through a short poly(A) tail and a PEG-amine linker at one end of said SPN sequence.
 61. The allergen detection agent of claim 60 wherein the solid substrate is selected from the group consisting of a magnetic particle, a glass slide, a silicon chip, a wafer or a microwell plate.
 62. The allergen detection agent of claim 61 wherein the solid substrate is a magnetic particle.
 63. The allergen detection agent of claim 62 wherein the complementary sequence is labeled with the fluorophore at one end; alternatively wherein the SPN sequence is labeled with the fluorophore at the free end which is not bound to the surface of the magnetic particle and the complementary sequence is labeled with a fluorophore quencher at one end; or alternatively wherein the complementary sequence is labeled with a first fluorophore at one end and the SPN sequence is labeled with a second fluorophore at the free end which is not bound to the surface of the magnetic particle.
 64. The allergen detection agent of claim 63 wherein the fluorophore is selected from the group consisting of Texas red, Alex 647, Cy3-FITC and Cy5.
 65. The allergen detection agent of claim 63 wherein the SPN and the complementary sequence is at a ratio of 1:2, or at a ratio of 1:3, or at a ratio of 1:4.
 66. The allergen detection agent of claim 65 wherein the SPN sequence is selected from the group consisting of nucleotide sequences presented by SEQ ID NOs.: 1-696.
 67. The allergen detection agent of claim 59 wherein the complementary sequence is immobilized to the surface of the solid substrate.
 68. The allergen detection agent of claim 67 wherein the complementary sequence binds to the SPN when the SPN sequence is not bound to the target allergen.
 69. The allergen detection agent of claim 68 wherein the solid substrate is magnetic particles, a glass slide, a silicon chip, a wafer or a microwell plate
 70. The allergen detection agent of claim 69 wherein the solid substrate is a glass slide.
 71. The allergen detection agent of claim 70 wherein one end of the SPN sequence is labeled with the fluorophore.
 72. The allergen detection agent of claim 70 wherein the complementary sequence is immobilized to the surface of the glass slide through a covalent reaction using an amine group, a thiol group, or a biotin-streptavidin linkage.
 73. The allergen detection agent of claim 72, wherein the surface of the glass slide is further coated with PEG polymers.
 74. The allergen detection agent of claim 70 wherein the complementary sequence is immobilized to the surface of the solid substrate by in situ synthesis that is mediated by a non-cleavable linker.
 75. The allergen detection agent of claim 74 wherein a spacer is attached to the non-cleavable linker which increases the space between the complementary sequences to facilitate hybridization of the SPN sequence.
 76. The allergen detection agent of claim 70 wherein the SPN sequence is selected from the group consisting of nucleotide sequences presented by SEQ ID NOs.: 1-696.
 77. A complex for detecting an allergen comprising: (a) an allergen binding signaling polynucleotide (SPN) comprising a nucleotide sequence selected from the group consisting of nucleotide sequences presented by SEQ ID NOs. 1-696; (b) a complement comprising a nucleotide sequence complementary to a region the SPN sequence wherein the complement comprises 5-20 nucleotide residues; and (c) a fluorophore.
 78. The complex of claim 77 wherein the SPN and the complement is at a ratio of 1:4, or at a ratio of 1:3, or at a ratio of 1:2.
 79. The complex of claim 78 wherein the complex is immobilized to the surface of a solid substrate, and wherein the solid substrate is selected from the group consisting of magnetic particles, a glass slide, a silicon chip, a wafer and a microwell plate.
 80. The complex of claim 79 wherein the complement sequence of the complex is immobilized on the surface of the solid substrate at one end, or alternatively the SPN sequence of the complex is immobilized on the surface of the solid substrate at one end.
 81. A method for detecting the absence, presence and/or quantity of an allergen of interest in a sample comprising: (a) obtaining and processing a sample suspected to contain the allergen of interest; (b) contacting the processed sample with a detection agent; (c) shaking the mixture and washing the mixture containing the allergen of interest and the detection agent; (d) detecting the SPN-allergen complexes; and (e) processing and analyzing the detection signals to determine the absence, presence, and/or the quantity of the allergen of interest in the sample, wherein the detection agent comprises a signaling polynucleotide (SPN) comprising a nucleotide sequence that specifically binds the allergen of interest, a complement comprising a nucleotide sequence complementary to the SPN sequence, a solid substrate and a fluorophore.
 82. The method of claim 81 wherein the solid substrate is selected from magnetic particles, a glass slide, a silicon chip, a wafer or a microwell plate.
 83. The method of claim 82 wherein the SPN sequence is immobilized to the surface of the solid substrate at one end.
 84. The method of claim 83 wherein the solid substrate is magnetic particles.
 85. The method of claim 84 wherein the complementary sequence is labeled with the fluorophore at one end; or alternatively wherein the SPN sequence is labeled with the fluorophore at the free end which is not bound to the surface of the magnetic particle and the complementary sequence is labeled with a fluorophore quencher at one end; or alternatively wherein the complementary sequence is labeled with a first fluorophore at one end and the SPN sequence is labeled with a second fluorophore at the free end which is not bound to the surface of the magnetic particle.
 86. The method of claim 85 wherein the SPN and the complement is at a ratio of 1:4, or at a ratio of 1:3, or at a ratio of 1:2.
 87. The method of claim 81 wherein the complementary sequence is immobilized to the surface of the solid substrate and wherein the SPN is labeled with a fluorophore at one end of the sequence.
 88. The method of claim 87 wherein the solid substrate is a glass slide.
 89. The method of claim 81 wherein the SPN comprises a nucleotide sequence selected from the group consisting of nucleotide sequences presented by SEQ ID NOs. 1-696. 